WO2001007584A1

WO2001007584A1 - Controlled electroporation and mass transfer across cell membranes

Info

Publication number: WO2001007584A1
Application number: PCT/US2000/019975
Authority: WO
Inventors: Boris Rubinsky; Yong Huang
Original assignee: The Regents Of The University Of California
Priority date: 1999-07-21
Filing date: 2000-07-20
Publication date: 2001-02-01
Also published as: US6403348B1; EP1196549B1; ATE463565T1; DE60044129D1; CA2378113A1; EP1196549A1; ES2341753T3; EP1196549A4; WO2001007584A8; JP2003505073A; CA2378113C

Abstract

Electroporation is performed in a controlled manner in either individual or multiple biological cells or biological tissue by monitoring the electrical impedance, defined herein as the ratio of current of voltage in the electroporation cell. The impedance detects the onset of electroporation in the biological cell(s), and this information is used to control the intensity and duration of the voltage to assure that electroporation has occurred without destroying the cell(s). This is applicable to electroporation in general. In addition, a particular method and apparatus are disclosed in which electroporation and/or mass transfer across a cell membrane are accomplished by securing a cell across an opening in a barrier between two chambers such that the cell closes the opening. The barrier is either electrically insulating, impermeable to the solute, or both, depending on whether pore formation, diffusive transport of the solute across the membrane, or both are sought. Electroporation is achieved by applying a voltage between the two chambers, and diffusive transport is achieved either by a difference in solute concentration between the liquids surrounding the cell and the cell interior or by a differential in concentration between the two chambers themselves. Electric current and diffusive transport are restricted to a flow path that passes through the opening.

Description

CONTROLLED ELECTROPORATION

AND MASS TRANSFER

ACROSS CELL MEMBRANES

FIELD OF THE INVENTION

This invention relates to the field of electroporation and mass transfer across cell membranes in general and the transport of ions across a cell membrane in particular

BACKGROUND OF THE INVENTION

Electroporation is a technique that is used for introducing chemical species into biological cells, and is performed by exposing the cells to an electπc potential that traverses the cell membrane While its mechanism is not fully understood, electroporation is believed to involve the breakdown of the cell membrane lipid bilayer leading to the formation of transient or permanent pores in the membrane that permit the chemical species to enter the cell by diffusion The electπc potential is typically applied in pulses, and whether the pore formation is reversible or irreversible depends on such parameters as the amplitude, length, shape and repetition rate of the pulses, in addition to the type and development stage of the cell As a method of introducing chemical species into cells, electroporation offers numerous advantages it is simple to use, it can be used to treat whole populations of cells simultaneously, it can be used to introduce essentially any macromolecule into a cell, it can be used with a wide vaπety of pπmary or established cell lines and is particularly effective with certain cell lmes, and it can be used on both prokaryotic and eukaryotic cells without major modifications or adaptations to cell type and ongin Electroporation is cuπently used on cells in suspension or in culture, as well as cells in tissues and organs

Electroporation is currently performed by placing one or more cells, in suspension or in tissue, between two electrodes connected to a generator that emits pulses of a high-voltage electπc field The pore formation, or permealization, of the membrane occurs at the cell poles, which are the sites on the cell membranes that directly face the electrodes and thus the sites at which the transmembrane potential is highest Unfortunately, the degree of permealization occurring in electroporation vanes with the cell type and also varies among cells m a given population Furthermore, since the procedure is performed in large populations of cells whose properties vary among the individual cells in the population, the electroporation conditions can only be selected to address the average qualities of the cell population; the procedure as currently practiced cannot be adapted to the specific characteristics of individual cells. Of particular concern is that under certain conditions, the electrical potential is too low for a cell membrane to become permeabilized, while under other conditions electroporation can induce irreversible pore formation and cell death. A high electric field, for example, may thus produce an increase in transfection efficiency in one portion of a cell population while causing cell death in another. A further problem with known methods of electroporation is that the efficiency of transfection by electroporation can at times be low. In the case of DNA, for example, a large amount of DNA is needed in the surrounding medium to achieve effective transformation of the cell. Many of the problems identified above are a consequence of the fact that the process of electroporation in both individual cells and tissues cannot be controlled in real time. There are no means at present to ascertain in real time when a cell enters a state of electroporation. As a result, the outcome of an electroporation protocol can only be determined through the eventual consequences of the mass transfer process and its effect on the cell. These occur long after the mass transfer under electroporation has taken place. These and other deficiencies of current methods of electroporation are addressed by the present invention.

Also relevant to the present invention are current techniques for the study and control of mass transfer across cell membranes. Knowledge of mass transfer across cell membranes in nature, both in cells that are functioning normally and in diseased cells, is valuable in the study of certain diseases. In addition, the ability to modify and control mass transfer across cell membranes is a useful tool in conducting research and therapy in modern biotechnology and medicine. The introduction or removal of chemical species such as DNA or proteins from the cell to control the function, physiology, or behavior of the cell provides valuable information regarding both normal and abnormal physiological processes of the cell. The most common method of effecting and studying mass transfer across a cell membrane is to place the cell in contact with a solution that contains the compound that is to be transported across the membrane, either with or without electroporation. This bulk transfer method does not permit precise control or measurement of the mass transfer across the membrane. The composition of the solution at specific sites is not known and is variable. In addition, when an electric field is present, the local field intensity will vary from one point to another.

Furthermore, the surface of the cell that is exposed to the solution is not well defined. Cell surface areas vary among cells in a given population, and this leads to significant differences among the cells in the amount of mass transfer. For these reasons, the amount of mass transfer achieved by bulk transfer processes is not uniform among cells, and the actual amount transferred for any particular cell cannot be determined

Attempts made so far to overcome the limitations of bulk transfer techniques include techniques for treating individual cells that include either the mechanical injection (microinjection) of chemical compounds through the cell membrane or electroporation with microelectrodes In injection techniques, the membrane is penetrated with a needle to deliver a chemical agent, localizing the application of the chemical agent to a small region close to the pomt of injection This requires manipulation of the cell with the human hand, a technique that is difficult to perform, labor-intensive, and not readily reproducible Electroporation with microelectrodes suffers these problems as well as the lack of any means to detect the onset of electroporation in an individual cell These problems are likewise addressed by the present invention

SUMMARY OF THE INVENTION

Devices, systems and particular methods are disclosed which make it possible to precisely monitor the movement of mateπals across a cell membrane The mformation gained from monitoring the movement of matenals across a cell membrane may be directly applied to deduce information with respect to the cell and/or its membrane Alternatively, the information obtained from monitoring may be applied m order to control the movement of mateπals across the cell membrane such as by controlling the application of electπcal current Devices and systems of the mvention make it possible to move charged molecules, and in particular lomc species, across a cell membrane and precisely monitor the occurrence of such When carrying out electroporation using the devices, systems and methods of the invention the information obtained from momtoπng the movement of the charged particles across the cell membrane is used to control the process of mass transfer across a cell membrane Specifically, the system is used to obtain measurements and changes m electrical impedance across a cell membrane while the mass transfer properties of the cell are changed by the application of electπcal current Thus, mformation obtamed on electπcal impedance changes brought by the application of electπcal cuπent are used, m real time, m order to control the movement of charged molecules across a cell membrane One aspect of the mvention is a method compπsmg creatmg an electπcal charge differential between a first pomt and a second point separated from the first point by an electncally conductive medium compπsmg a biological cell A first electπcal parameter between the first and second points is then measured A second electπcal parameter is then adjusted based on the measuring of the first electπcal parameter The first electπcal parameter may be any parameter such as one selected of the group consistmg of current, voltage and electncal impedance The second electπcal parameter may be any parameter (the same as or different from the first electncal parameter) such as one selected from the group consistmg of current, voltage or a combination of current and voltage

In a preferred embodiment the method further mcludes placmg a mateπal m the electπcally conductive medium, and adjustmg the second electπcal parameter m order to move the matenal mto the biological cell The matenal placed within the electπcally conducted medium may be any mateπal such as a pharmaceutically active compound or drug, a nucleotide sequence, a fluorescent dye, or a crystal which is specifically designed to effect the cell in a desired manner In accordance with the method various conditions are adjusted so that the electncal potential between the two pomts is sufficiently high so as to cause the cell to be permeabilized However, the conditions between the two pomts are further adjusted so that electroporation is reversible and as such does not cause cell death unless that is a result specifically bemg sought

In another aspect of the mvention the electroporation is not earned out for the purpose of movmg matenal mto or out of a cell but rather to analyze the cell or group of cells and provide information or diagnosis of the tissue or individual which contams the tissue In accordance with this method an electncal charge differential is created between a first pomt and a second pomt separated from the first pomt by an electncally conducted medium compπsmg a biological cell A first electncal parameter is then measured between the first and second pomts The measuring of the first electrical parameter is then analyzed in order to determine a character of the cell and m particular a charactenstic of a membrane of the cell The first electncal parameter may be any parameter and is preferably selected from the group consisting of current, voltage and electπcal impedance A second electπcal parameter is preferably adjusted in a manner which effects the membrane of the cell or cells present m the medium and the second electncal parameter is any parameter but preferably selected from cuπent, voltage or a combmation of both

Another aspect of the mvention is the device which is preferably compnsed of a first electrode, a second electrode, a source of electπcity which may later be connected to the electrodes but is optionally present when the device is sold The device further mcludes a means for hindering the flow of electπcal current between the first and second electrodes except for electπcal cuπent flow through a defined route Further, the device mcludes a means for measuring an electπcal parameter such as current, voltage or electπcal impedance through the defined route and a means for adjusting the source of electricity based on the measured electrical parameter. The means for hindering electrical current flow is preferably comprised of a non- conductive material and defined route comprised of one or more openings each with a diameter less than that of a biological cell so that a cell can fit within the defined route and have a current flow through but preferably not around the cell.

The device and systems of the invention can be used within the method in order to move a wide range of materials into or out of the biological cell in order to obtain a desired result. The process can be carried out on an individual cell, a group of cells, cells within a cell culture or within a living organism, e.g. cells within invertebrates and vertebrates including mammals as well as in plants. When carrying out the process on a plurality of cells (e.g. a tissue) a process of imaging the tissue and adjusting electrical current in real time based on images may be used. An imaging technology which may be applied is electrical impedance tomography (EIT). This technology relies on differences in bioelectrical attributes within the body or an organism (e.g. a human) to produce an image. In the method of the invention EIT images can be used in the same manner as the measuring step is used when the process is carried out on a single biological cell. In essence, the EIT technology makes it possible to "see" the effect of increased electrical current flow resulting from electroporation thereby providing information which can be used to precisely adjust the flow of electrical current so that cell membranes are permeabilized while not permanently disrupted. Another aspect of the invention is a method which comprises sending an electrical current between a first point and a second point separated by the first point by an electrically conductive medium comprising tissue. The tissue may be present within a living organism such as a vertebrate or invertebrate and specifically includes mammals and humans. After the cuπent is sent an image of the tissue is created wherein the image is based on an electrical parameter such as the electrical impedance of the tissue. Using the image as a guide an electrical parameter is adjusted in order to obtain a desired degree of electroporation of biological cells in the tissue. Electroporation will change electrical impedance and that change can be visualized on the image created. The electrical parameter adjusted may be any parameter such as current, voltage or a combination of both. In a preferred embodiment a material is placed in the electrically conducted medium such as being injected into the tissue and the adjustment of the current is carried out, based on the image, in a manner so as to move the material into biological cells of the tissue. The image created is preferably an impedance image created from known current inputs and measured input voltage using a reconstruction algorithm. The impedance image may be created from a known voltage input, a measured current input, or combination of known voltage input and measured current input.

A device for carrying out this method is another aspect of the invention which device includes a means for creating an electrical current across an electrically conducted medium. The device further includes a means for analyzing a first electrical parameter of the electrically conductive medium in order to create an image and a means for adjusting a second electrical parameter based on the image to obtain a desired degree of electroporation of biological cells in the electrically conductive medium. The first electrical parameter is preferably electrical impedance and the second electrical parameter is preferably selected from the group consisting of current, voltage or a combination of both. The cuπent is preferably created by a plurality of electrodes positioned about an area of tissue upon which the electroporation is to be carried out.

The present invention arises in part from the discovery that the onset and extent of electroporation in a biological cell can be correlated to changes in the electrical impedance (which term is used herein to mean the ratio of current to voltage) of the biological cell or of a conductive medium that includes the biological cell. An increase in the cuπent-to-voltage ratio across a biological cell occurs when the cell membrane becomes permeable due to pore formation or because of cell damage or other modes of cell membrane poration. Likewise, a decrease in the cuπent-to-voltage ratio through a flowing conductive fluid occurs when the fluid draws a biological cell into the region between the electrodes in a flow-through electric cell. Thus, by monitoring the impedance of the biological cell or of an electrolyte solution in which the cell is suspended, one can detect the point in time in which pore formation in the cell membrane occurs, as well as the relative degree of cell membrane permeability due to the pore formation. This information can then be used to establish that a given cell has in fact undergone electroporation, or to control the electroporation process by governing the selection of the electrical parameters of the process e.g. the voltage magnitude. This discovery is also useful in the simultaneous electroporation of multitudes of cells in a cell culture or in vertebrates, invertebrates or plants. Specific embodiments apply the invention to mammals including humans. The process provides a direct indication of the actual occuπence of electroporation and an indication of the degree of electroporation averaged over all the cells being subjected to the process. The discovery is likewise useful in the electroporation of biological tissue (masses of biological cells with contiguous membranes) for the same reasons.

The benefits of this process include a high level of control over the onset and degree of electroporation, together with a more detailed knowledge of the occuπence and degree of permeability created in particular individual cells or cell masses. When applied to individual cells or to a succession of individual cells, this process assures that the individual cells are indeed rendered permeable and are indeed transformed by the introduction of chemical species The process also offers the ability to mcrease the efficiency of electroporation by avoidmg vaπations m the electncal environment that would destroy some cells while havmg an insufficient effect on others

The invention can be understood by descπbmg a simple embodiment which mvolves the use of an electπcal device or system m which a biological cell can be placed and that contains a barπer that directs the electnc current flow and hence the ion flow through a flow path that passes through the biological cell while permitting substantially no electnc current to bypass the biological cell In some of these embodiments, the mvention mvolves the use of an apparatus containing two liquid-retaining chambers separated by a barπer that is substantially impermeable to an electnc current The bamer contams an openmg that is smaller than the biological cell such that the biological cell once lodged in the openmg will plug or close the openmg To achieve electroporation, the biological cell is secured over the openmg by mechanical, chemical and/or biochemical means, preferably m a reversible manner so that the biological cell can later be removed without damage to the biological cell Once the biological cell is secured over the openmg, a voltage is imposed between the two chambers and across the biological cell residmg in the openmg The passage of cuπent between the chambers is thus restπcted to a path passmg through the openmg and hence through the biological cell By momtoπng the current-voltage relation m the electnc cell, the onset of electroporation is detected and the degree of pore formation is controlled, to both assure that electroporation is occurring and to prevent excessive pore formation and cell death The user is thus afforded a highly precise knowledge and control of the condition of and the flux across the biological cell membrane

In another senes of embodiments, this mvention is useful m the diffusive transport of chemical species mto or out of a biological cell In these embodiments, the cell is again divided mto two chambers separated by a barner, and the biological cell is lodged across an openmg in the barner m such a manner that the passage of liquid around the cell from one chamber to the other is substantially prevented A liquid solution of the species to be introduced mto the biological cell is placed m one or both of the chambers The concentration of the species m the solution differs from that in the cell (either higher or lower, dependmg on whether one seeks to introduce or remove the species from the cell), or the concentration in one chamber differs from that in the other chamber

In prefeπed methods of applying this mvention to diffusive transport, the solutions in the two chambers differ m concentration such that the dnvmg force for the diffusive transport is between the two chambers themselves rather than between the chambers and the mteπor of the biological cell Knowledge and controlled monitoring of the concentrations m each of the two chambers on a peπodic or contmuous basis as the diffusion proceeds, together with the precise knowledge of the dimensions of the openmg, enables the user to precisely observe and control the rate and amount of the species that enters the cell The diffusion time can be controlled by imposmg stepwise changes m the concentrations m either or both of the chambers, thereby imposmg or removing the concentration differential An application of particular mterest is the combmation of this type of diffusive transport of a chemical species with controlled electroporation as descπbed in the preceding paragraph In addition to bemg useful in connection with electroporation technology the present mvention can provide valuable mformation relatmg to a cell or group of cells or tissue containing a group of cells by monitoring electπcal impedance and thereby providmg mformation regarding the integnty of a cell membrane Specifically, measurements are earned out regarding the movement of charged particles across a cell membrane These measurements are related to the amount of electncal cuπent needed to carry out the diffusion across a cell membrane The mformation obtained can be analyzed directly or compared to previous measurements of a same tissue or measurements earned out on diseased or normal tissue thereby providmg an indication of the amount of change which has occurred m the tissue bemg measured (based on an earlier measurement of the same tissues) or the amount of vaπance between the tissue bemg measured and tissue with impaired cell membranes (e g diseased cells) or a normal cell or tissue The method is earned out m a manner similar to that used for conducting electroporation However, no mateπal needs to be added to the medium suπounding the cells The device is similar m that it is divided mto two portions with a positive electrode on one side and a negative electrode on another side separated by a barπer with the cells bemg positioned along openmgs on the barner m a manner which allows for the passage of charged particles through the cell and through the openmg m the barπer from one electrode to another The bamer hinders or completely eliminates the flow of charged particles except through the openmgs The measurement of electncal impedance between the electrodes make it possible to distinguish between cells with an mtact membrane and cells with impaired membranes By more precisely carrying out the measurements it is possible to make determmations with respect to the integnty of a normal cell membrane relative to an impaired (e g diseased) cell membrane

Each of the various embodiments of this mvention may be used with two or more (l e a plurality of) biological cells simultaneously, or cell masses such as m tissue which may be in an animal or plant during the process The apparatus descnbed above can be adapted for use with two or more biological cells by arranging the barrier such that the current or diffusive transport will be restricted to a flow path that passes through all of the cells while preventing bypass around the cells. A further application of the concepts of this invention is the electroporation of biological cells suspended in a flowing liquid. Electrodes are placed in fixed positions in the flow channel, and a voltage is imposed between the electrodes while current passing between the electrodes is monitored. Biological cells entering the region between the electrodes will lower the current, the impedance serving as an indication of the presence of one or more cells in the region, and optionally also as a signal to initiate the application of a higher voltage sufficient to achieve electroporation. A further application of the device, system and method of the invention is the electroporation of biological cells present within a tissue which tissue may be present within a living organism such as a mammal. Electrodes are placed in fixed positions within the tissue, and voltage is applied between the electrodes while current passing between the electrodes is monitored. Biological cells with intact membranes in the region between the electrodes will increase the electrical impedance. Accordingly, a measurement of the electrical impedance provides an indication of the presence of one or more cells in the region. Electroporation will decrease the measured amount of impedance. When the process is carried out on a tissue then the measurement of electrical impedance is a statistical average of the cells present between the electrodes. Electroporation methodology of the invention can be carried out on tissue in a living organism using an imaging technology which makes it possible to determine when (and preferably to some extent the degree) cell membranes are transformed so as to allow the flow of electrical current through their membranes. The preferred imaging technology is electrical impedance tomography (EIT) which provides a changing image created from information on differences in bio-electrical attributes of the tissue being imaged. A typical EIT image is acquired by injecting electrical currents into the body and measuring the resulting voltages through an electrode array. An impedance image is then produced from the known current inputs and the measured voltage data using a reconstruction algorithm. EIT is particularly appropriate for the implementation of the invention in tissue because it actually maps electrical impedances. Therefore, the region of tissue that will undergo electroporation and in which, consequently, the equivalent electrical impedance of the cells will change will be imaged by EIT. The image is used to adjust the electrical parameters (e.g. flow of electrical current) in a manner which allows electroporation to occur without damaging cell membranes. Among the advantages that this invention offers relative to the prior art are the ability to treat cells individually and to adapt the treatment conditions to the needs of individual cells. In embodiments where voltage is applied, the monitoring of the impedance affords the user knowledge of the presence or absence of pores and shows the progress of the pore formation and whether iπeversible pore formation that might lead to cell death has occurred.

An advantage of the barrier-and-opening apparatus is the high sensitivity of the signal to noise ratio by virtue of its restriction of the cuπent to a current flow path passing through the opening.

A still further advantage is the ability of the apparatus and method to be integrated into an automated system whereby the condition of each cell is monitored by instrumentation and individual cells are lodged in the opening and then removed at times governed by the monitored conditions.

An aspect of the invention is a method of controlling electroporation of biological cells in real time by adjusting an electrical parameter (e.g. voltage and/or current) applied to a system based on real time measurements of changes in cuπent detected.

A feature of the invention is that the general concepts can be applied to carry out electroporation on a cell, multiple cells, a tissue or areas of tissues in a living animal.

An advantage of the invention is that a precise amount of electroporation can be obtained and cell damage avoided by controlling any given electrical parameter (e.g. current and/or voltage) applied based on real time measurements of changes in current which relates to the amount of electroporation being obtained.

Another advantage of the invention is that it can be used to transfect cells with nucleotide sequences without the need for packaging the sequences in a viral vector for delivery, thereby avoiding the cellular specificities of such vectors. Still other advantages are that the process can be carried out relatively quickly with a relatively low degree of technical expertise.

Yet another advantage is that the process can be used to transfect cells without generating an immune response.

Still another advantage is that the process is not limited by the size of the DNA (i.e. the length of the DNA sequences) and the amount of DNA brought into a cell can be controlled.

Another feature of the invention is that imaging technologies such as EIT can be used to detect changes in impedance in a volume of cells. Another feature of the mvention is that it can use EIT in order to map impedance of an area of tissue and thereby detect changes m cell impedance m a volume of cells to adjust any given electπcal parameter (e g current flow and/or voltage) to obtain desired electroporation

These and further features, advantages and objects of the mvention will be better understood from the descπption that follows

BRIEF DESCRIPTION OF THE DRAWINGS

FIG 1 is a cross section of a microdiffusion device useful m the practice of the present invention for mfusmg a biological cell with a chemical species without the assistance of an electncal current to effect electroporation FIG 2 is a cross section of a microelectroporation device useful in the practice of the present mvention for achievmg pore formation in a biological cell, and optionally for mfusmg the cell with a chemical species with the assistance of electroporation

FIG 3a is a longitudinal cross section of an electroporation device m accordance with this mvention, designed for a mobile suspension of biological cells FIG 3b is a transverse cross section of the device shown in FIG 3a

FIG 4 is a plot of current vs voltage m a senes of electroporation expenments conducted usmg a microelectroporation device of the structure similar to that of FIG 2

FIGS 5a, 5b, 5c, and 5d are plots of current vs voltage m a further senes of electroporation expenments conducted usmg a microelectroporation device similar to that of FIG 2

FIG 6a shows cuπent flow around cells pnor to electroporation and FIG 6b shows electπcal current flow through cells after (during) electroporation

FIG 7 shows a typical electncal impedance tomography (EIT) system for use with the mvention FIG 8a is an image of current flow through cells with irreversible electroporation and FIG 8b is an image of cuπent flow through cells with reversible electroporation

FIG 9 is a graphic schematic view of a finite element mesh showing a circular region of tissue bounded by electrodes (dark dots) — the domam has two different impedances FIG 10 schematically shows typical electrode configuration, measured electncal vaπables and equipotential lines m a circular domam having an inclusion with a different electncal impedance FIG. 11 shows an actual image in the top left whereas the impedance mapping is shown in the bottom right which shows differential impedance mapping.

DESCRIPTION OF THE INVENTION AND SPECIFIC EMBODIMENTS Before the present devices and methods including methods for carrying out electroporation are described, it is to be understood that this invention is not limited to particular methods and devices described, as such may, of course, vary. It is also to be understood that the terminology used herein is for the purpose of describing particular embodiments only, and is not intended to be limiting, since the scope of the present invention will be limited only by the appended claims.

Where a range of values is provided, it is understood that each intervening value, to the tenth of the unit of the lower limit unless the context clearly dictates otherwise, between the upper and lower limits of that range is also specifically disclosed. Each smaller range between any stated value or intervening value in a stated range and any other stated or intervening value in that stated range is encompassed within the invention. The upper and lower limits of these smaller ranges may independently be included or excluded in the range, and each range where either, neither or both limits are included in the smaller ranges is also encompassed within the invention, subject to any specifically excluded limit in the stated range. Where the stated range includes one or both of the limits, ranges excluding either or both of those included limits are also included in the invention.

Unless defined otherwise, all technical and scientific terms used herein have the same meaning as commonly understood by one of ordinary skill in the art to which this invention belongs. Although any methods and materials similar or equivalent to those described herein can be used in the practice or testing of the present invention, the prefeπed methods and materials are now described. All publications mentioned herein are incorporated herein by reference to disclose and describe the methods and/or materials in connection with which the publications are cited.

It must be noted that as used herein and in the appended claims, the singular forms "a", "and", and "the" include plural referents unless the context clearly dictates otherwise. Thus, for example, reference to "a biological cell" includes a plurality of such biological cells and reference to "an electrode" includes reference to one or more electrodes and equivalents thereof known to those skilled in the art, and so forth. The publications discussed herein are provided solely for their disclosure prior to the filing date of the present application. Nothing herein is to be construed as an admission that the present invention is not entitled to antedate such publication by virtue of prior invention. Further, the dates of publication provided may be different from the actual publication dates which may need to be independently confirmed.

DEFINITIONS

The term "electrode" is intended to mean any conductive material, preferably a metal, most preferably a non-corrosive metal that is used to establish the flow of electrical cuπent from that electrode to another electrode. "Electrically conductive" means for transmitting electrical current that can be refeπed to in any manner, e.g. cuπent or voltage. Electrodes are made of a variety of different electrically conductive materials and may be alloys or pure metals such as copper, gold, platinum, steel, silver, silver chloride, and alloys thereof. Further, the electrode may be comprised of a non-metal that is electrically conductive such as a silicon-based material used in connection with microcircuits. Typical electrodes used in tissue electroporation are preferably rod-shaped, flat plate-shaped or hollow needle-shaped structures. Electrodes may be used to deliver electrical current continuously or to deliver pulses. The electrodes may be very application-specific and be comprised of parallel stainless steel plates, implanted wires, needle pairs and needle arrays. Those skilled in the art will design specific electrodes that are particularly useful in connection with the desired results of obtaining electroporation in accordance with the present invention.

The term "tissue" shall mean a plurality of cells. The cells may be of the same or of a number of different types. These cells are preferably organized to carry out a specific function. Tissue includes tissue present within a living organism as well as removed tissue and may refer to in vivo or in vitro situations. Further, the tissue may be from any organism including plants and animals or a tissue developed using genetic engineering and thus be from an artificial source. In one embodiment the tissue is a plurality of cells present within a distinct area of a human.

The terms "device" and "electroporation device" are used interchangeably here for describing any a device as disclosed and described throughout. The device preferably includes a first electrode and a second electrode wherein the first and second electrodes are connected to a source of electricity in a manner so as to provide the electrodes with positive and negative charges respectively. The device also preferably includes a means for hindering the flow of electricity between the two electrodes except through one or more specific openings. For example the means for hindering flow can be a non-conductive material which has one or more openings therein wherein the openings are designed so as to specifically hold a biological cell or group of biological cells. Thereby the electrical current must flow through the opening and through the cells to the other electrode. The device also preferably includes a means for measuring the flow of electrical current between the electrodes. The means for measuring can include a volt meter, amp meter or any device known to those skilled in the art which is capable of measuring the flow of electrical current in any manner. Further, the device preferably includes a means for adjusting the amount of electrical cuπent flow between the electrodes. Thereby the voltage, current or other desired parameter of electrical current flow can be specifically adjusted based on the measured flow so as to obtain optimum electroporation of the cell or cells positioned between the electrodes. When the term "electroporation" is used it does not necessarily mean that the device is being used in order to move a compound such as a drug or DNA sequence into a cell. The terms "power source", "source of electricity" and the like, are used interchangeably herein to describe any means for providing electrical power, current or voltage thereby creating a flow of electrical cuπent between the electrodes. The device preferably is capable of providing for a controlled mode and amplitude and may provide constant DC current or AC cuπent, provide pulse voltage or continuous voltage. Prefeπed devices are capable of exponentially decaying voltage, ramp voltage, ramped cuπent, or any other combination. For example, a power supply may be used in combination with a chip of the type used in connection with microprocessors and provide for high-speed power amplification in connection with a conventional wall circuit providing alternating cuπent at 110 volts. The pulse shape may be generated by a microprocessor device such as a Toshiba laptop running on a Lab View program with output fed into a power amplifier. A wide range of different commercially-available power supplies can provide the desired function. The electrical potential delivered for electroporation is usually quoted in terms of the voltage gradients that develop in the affected region that is defined in units of V/cm developed in the tissue. Ranges include a range of 10 V/cm to 100,000 V/cm or more preferably 100 V/cm to 10,000 V/cm. However, the range is amplification-specific and can be extended outside the range for any desired application. Electrical pulses range from microseconds to milliseconds in general. However, other ranges of pulsing may be utilized depending on the desired results. INVENTION IN GENERAL While this invention extends to a variety of structures, methods, and applications, this portion of the specification will illustrate certain specific structures and methods in detail, from which the concepts of the invention as a whole will become apparent. A wide range of different devices and system can be used to carry out the method of the invention. The device must be comprised of a first electrode having a first voltage and a second electrode having a second voltage. Further, the device will comprise a means for detecting charged particle flow between electrodes and a means for varying the electrical current between electrodes based on data obtained by detecting changes in charged particle flow between electrodes. Preferably the device is further comprised of a component that prevents or substantially reduces charged particle flow between electrodes except for flow occurring through one or more biological cells positioned between the first and second electrodes.

Any desired material can be added to the medium in order to move that material into a cell which is present in the medium. Further, the invention does not necessarily include a process step of including a material into the medium which is to be brought into a cell. The process can be carried out merely to determine changes which occur in a cell membrane based on the electrical current applied. That information can be valuable to determine characteristics about the cell or group of cells present in the medium and, specifically, can be used to compare with information on normal and diseased cells or to determine the differences between previously tested cells and those currently being tested.

The first structure that will be discussed is an electroporation cell with an internal support to hold a single biological cell and an internal barrier that restricts the electric current flow in the electric cell to a flow path that passes through the biological cell. When no voltage is applied, the structure can be used for diffusive transport alone, unassisted by voltage-induced pore formation.

The configuration of the barrier, and the two chambers in embodiments that include two chambers, is not critical to the invention, and can vary widely while still serving the purposes and advantages of the invention. Since biological cells are microscopic in size, however, the preferred type of apparatus for the practice of this invention in each of its various forms is one in which the structure as a whole and/or its chambers are the size of electronic chips, fabricated by microfabrication techniques such as those used in electronic chip manufacture. It is further prefeπed that the chambers are constructed as flow-through chambers to allow the passage of the liquids in continuous flow, intermittent flow, or flow at the direction of the user, and to allow changes in the concentrations, pressure, and other conditions as needed to achieve close control over the passage of species across the biological cell membrane. Accordingly, a preferred structure and method of manufacture of the apparatus are those that involve the formation of the apparatus in layers or platelets with appropriate openings that form flow passages when the layers or platelets are bonded together. Flow-through chambers offer the advantage of permitting the successive entry and removal of individual cells so that large numbers of cells can be treated in succession. Flow- through chambers also permit replenishment of solute-depleted solutions so that concentration gradients can be continuously maintained when desired. A further function that can be served by flow-through chambers is the increase and decrease of pressure, a function that is useful for various purposes as described below.

The support for the biological cell in this structure can be any structure that secures the biological cell in a fixed position and that allows the passage of electric current. The most convenient support is an opening in the barrier. Securement of a biological cell over the opening serves to close, seal or plug the opening, thereby directing the passage of electric current, diffusive transport, or both, through the cell and eliminating or minimizing leakage around the cell. A convenient mechanical means of achieving this is to impose a pressure differential across the opening in a direction that will press the cell against the opening. The diameter of the opening will be smaller than that of the cell, and the cell upon entering the apparatus will pass into one of the two chambers. By increasing the pressure in the chamber in which the cell resides, or lowering the pressure in the other chamber, the cell will be forced against the opening, closing it off. Once the procedure is completed, the cell is readily released from the opening by equalizing the pressures in the two chambers or by reversing the differential such that the higher pressure is in the chamber other than the chamber in which the cell was introduced. The flow of liquid in the chamber in which the cell was introduced will then remove the cell from the opening, exposing the opening for another cell.

An alternative method of sealing the opening with the cell is by the use of a coating on the barrier surface, or over the rim of the opening, of a substance that binds to the cell membrane. Since biological cell membranes are negatively charged, the coating may be a substance that bears a positive charge, such as polylysine, polyarginine, or polyhistidine. The biological cell can be directed to the opening by a pressure differential across the opening, and held in place by the coating. Once the procedure is completed, the cell can be released from the coating by momentarily increasing the flow rate of the liquid in the chamber on the cell side of the opening, or by imposing a reverse pressure differential across the opening to urge the cell away from the opening. The size of the opening is not critical to the invention provided that the opening exposes sufficient surface area on the cell membrane to achieve the desired degree of either mass transfer, the passage of an electric current, or both, within a controllable and economically reasonable period of time. The optimal size will thus vary with the particular cells being treated or studied. In general, the opening is preferably circular or approximately circular in shape, and depending on the cell size, preferably ranges in diameter from about 1 micron to about 100 microns, more preferably from about 1 micron to about 50 microns, and most preferably from about 2 microns to about 20 microns. The barrier in which the hole is formed and which separates the two chambers is preferably of a rigid dielectric material that is impermeable to both water and solutes and that will hold a pressure differential sufficient to secure a cell against the opening. For devices that are manufactured by microfabrication techniques, a convenient material for the barrier is silicon nitride. Other materials that will serve equally well will be readily apparent to those skilled in the art.

A further feature of preferred embodiments of this invention is the use of apparatus made of transparent materials. This enables the user to observe cell interiors and the processes of micro diffusion and microelectroporation through a microscope as they occur.

ELECTROPORATION USED IN IN VIVO THERAPY The electroporation techniques of the present invention are useful in connection with treating, analyzing or diagnosing an organism including mammals and humans in need of treatment. In general, treatment may be carried out by injecting a material continuously or in a rapid bolus into an area of tissue to be treated. Electrodes are placed adjacent to the tissue and cuπent or voltage are applied and measured continuously in order to determine when the desired level of electroporation is obtained thereby making it possible to move the injected material into the cells of the tissue being treated.

The pharmaceutically active compound that is injected may be a conventional drug normally referred to as a small molecule or be a protein or nucleotide sequence that encodes a protein. Further, the composition injected into the tissue may be administered before, during or even after the application of electrical pulses from the electroporation device. The overall goal of the process is to provide for the opening of pores via electroporation and thereby introduce the compounds into the cells which compounds would not normally penetrate the cell membrane. For example, it is possible to introduce bleomicyn or various gene constructs and/or plasmids into cells of the tissue being treated. This is accomplished by generating electrical potentials and currents across the cells within the tissue to treated wherein the electrical potentials are generated as electncal pulses It is preferable to utilize a plurality of electrodes as opposed to a smgle electrode in order to generate the pulses

An example of a useful electrode design is one that is compnsed of two flat steel stnps 10 mm m width and 0 6 mm m thickness The electrodes are spaced at a fixed distance of approximately 6 to 7 mm from each other A second electrode design is compnsed of two to as much as eight flat steel squares of 20 mm The electrodes are connected to a PS 15 electropulsator Pulses can be delivered by placing the electrodes on the skm with the flat side on the skm or by placmg the electrodes around skm tumors Skm contact can be achieved by the use of mateπals conventionally used m connection with performing electrocardiographs such as electro-conductive gels or salme In order to carry out the procedure a patient can receive one or a plurality of pulses and preferably receives a plurality of pulses Different configurations can be designed in order to carry out electroporation of tissue mside an organism such as mside a human body, l e without applying electrodes outside the skm Such configurations can be compnsed of needle arrays that compnse a plurality of needle electrodes As an example the positive and negative electrodes can each be compnsed of six or more needles that are 0 5 mm m diameter and compnsed of stainless steel, 1 cm in length connected to a BTX 820 pulse generator The electrodes can be inserted m parallel mto the tissue around the cells to be affected by electroporation The electrodes can be positioned m circles of various diameters ranging from 5 mm to 1 cm Voltage electrode ratio m the range of approximately 1300 V/cm can be used Although any number of pulses can be delivered it is preferable to begm the process by delivermg approximately six pulses m one second intervals with a pulse width of 100 microseconds The present invention is particularly desirable m connection with electroporation of tissue m that the method can determine whether electroporation is occurπng without the use of dyes and tags in order to track the mateπal bemg brought mside the cell As shown m FIGS 6a and 6b the electrical cuπent can flow around the cells (FIG

6a) or through the cells (FIG 6b) after electroporation has taken place The process of the mvention makes it possible to determine the point when the transition is occurπng between what is shown m FIG 6a and what is occurring m FIG 6b and further makes it possible to prevent the occurrence of meversible effects on the cell membranes As shown m FIG 8a the electroporation can be earned out to such a great extent that cell membranes are damaged thereby resulting in meversible effects on the cells In general, this is undesirable However, by modulating the amount of electπcal cuπent it is possible to obtain electroporation without significant damage to the cell membranes thereby obtaining a reversible situation as shown m FIG 8b As shown m FIGS 6a and 6b cells create electncal impedance and the present mvention relates to precisely determining the degree of that electncal impedance and adjusting current so as to obtain desired results with respect to electroporation However, when large numbers of cells are mvolved such as m a tissue it may be desirable to use other mechanisms for measunng other effects of the cuπent m creatmg electroporation on a plurality of cells m the tissue Electncal impedance is a measurement of how electncity travels through a given mateπal Every mateπal has a different electncal impedance determined by it's electπcal composition Some matenals have high electπcal impedance and others have low electπcal impedance Breast tissue which is malignant (cancerous) has much lower electπcal impedance (conducts electncity much better) than normal tissue or a benign (non-cancerous) tumor

Impedance is a measurement of the degree to which an electπcal circuit resists electncal-cuπent flow when voltage is impressed across its terminals Impedance expressed m OHMS, is the ratio of the voltage impressed across a pair of terminals to the current flow between those terminals In direct-current (DC) circuits, impedance coπesponds to resistance In alternating current (AC) circuits, impedance is a function of resistance, inductance, and capacitance Inductors and capacitors build up voltages that oppose the flow of current This opposition is referred to as reactance, and must be combmed with resistance to define the impedance The resistance produced by inductance is proportional to the frequency of the alternating cuπent, whereas the reactance produced by capacitance is mversely proportioned to the frequency

The basic concepts descnbed above are utilized m the basic aspects of the present mvention and are also applicable to descnbmg electncal impedance imagmg also referred to as electπcal impedance tomography (EIT) It should be noted that a number of different terminologies may be used to describe the same technique and those mclude applied potential tomography (APT) These imagmg technologies make it possible to produce images based on the spatial vanation of the electncal properties of the biological tissue Techniques such as APT and EIT could be utilized to carry out the mvention m connection with tissue The applied potential tomography (APT) relies for its physical basis on the measurement of a potential distribution on a surface of a biological matenal, when an electncal cuπent is applied between two points of its surface Other researchers have utilized the techmque and refeπed to it as electncal impedance imagmg, conductivity imagmg, electrical impedance tomography, etc Herein, the technology is generally refeπed to as EIT or electncal impedance tomography Accordingly, within the remamder of the disclosure the technology is refeπed to only as EIT technology and an example of such is shown within Example 3 below Those skilled in the art will contemplate different means of determining changes m electncal cuπent upon reading this disclosure A preferred method for determining such when carrying out the mvention on tissue is to use imagmg technology and specifically electπcal impedance tomography (EIT) which monitors and analyzes differences m bio-electncal attributes of the sample bemg monitored m order to produce an image The EIT technology can be used in connection with the present mvention by creating an EIT image and usmg that image to adjust current flow to obtain desired results Specifically, the EIT image is created by injecting electncal currents mto the tissue and measunng the resulting voltages through an electrode array This makes it possible to produce an impedance image from the known cuπent mputs and the measured input voltage data usmg a reconstruction algonthm The use of EIT technology is particularly desirable m connection with the present invention as applied to tissue m that EIT imagmg provides a map of electπcal impedances The map of electncal impedances essentially allows the user to visualize when electroporation is beginning When electroporation begins the user can stabilize the amount of current bemg applied and thereby avoid applymg so much cuπent as to result m irreversible damage to cells as shown m FIG 8a The EIT technology makes it possible for the region of tissue undergoing electroporation to be visualized based on changes in equivalent electrical impedance of the cells within tissue bemg monitored

FIG 7 shows a conceptual view of an EIT system bemg used to carry out a process of the present mvention on tissue 71 A current source 72 is controlled by a signal generator 73 and is used to dπve an electπcal current mto the tissue sample 71 through a pair of computer controlled multiplexers 74 and 75 which lead to a differential amplifier 76 and demodulator 77 The measured signals are compared to the ongmal m order to record amplitude and phase data for later image construction The controlling computer 78 typically chooses which pair of electrodes will mject cuπent while readmg the remaining electrode voltages There are a number of different hardware configurations which can be utilized m connection with the present invention The EIT system as shown m FIG 7 is generally refeπed to as a senal system because of it's smgle cuπent source and measurement amplifier Varying degrees of parallelism (multiple current sources and voltage measunng amplifiers) have been utilized in other systems thereby mcreasmg the flexibility and speed of the cuπent injection system Reconstruction algonthms are used in order to take the voltage measured on an outer surface of a region of interest m the body (the injected current data) and mformation relatmg to the electrode geometry, and produce an image which represents spatial tissue impedance tissue distπbution mside the region of the tissue 71 There are a number of methods which can be used to create an impedance image Static imaging is the production of an absolute impedance distribution. Cook, R. D. et al. ACT3: a high speed, high precision electrical impedance tomography. IEEE, Trans. Biomed. Eng. 41, 713-22 (1994). Differential imaging methods produced distributions based on differences between two data sets. Barber, D. C. in Advances in Biomed Eng. (ed. Benek in, W., Thevenin, V.) 165-173 (IOS Press, Amsterdam, 1995). This type of technique provides an image of how the impedance distribution has changed from one baseline measurement. Multi frequency impedance imaging takes advantage of the frequency dependence of tissue impedance. Groffiths, H. The importance of phase measurement in electrical impedance tomography. Physics in Medicine and Biology 32, 1435-44 (1987). Quasi-static images can be produced using the above differential technique with a low frequency image used as the baseline. Accordingly the system makes it possible to produce a type of static imaging without the difficulties of true static imaging.

In order to provide for reconstruction and thus and image , a mathematical model of how the current behaves in the tissue is used. In general a model governing current flow in EIT is provided by the well-known Poisson equation. The type of mathematical analysis that is needed in EIT image reconstruction as well as many other medical imaging technologies, belongs to a general class known as boundary value problems. There are a number of different methods of solving boundary value problems. However, these problems can all be classified into either analytical or numerical iterative techniques and those skilled in the art can apply such in order to carry out the present invention. The vast majority of reconstruction algorithms cuπently in use employ iterative numerical solutions to the Poisson equation. Most iterative numerical approaches attempt to solve the boundary value problem by guessing an impedance distribution in the tissue and repeatedly solving the forward problem (finding the voltage and current densities given an impedance distribution) and adjusting the impedance guesses correspondingly, until the voltage and cuπents measured fit those calculated. The forward problem must be solved numerically and is usually done so using finite element or finite difference schemes. The FEM is a very powerful and popular method of forward problem solution, and because of this, tends to dominate engineering solutions across many interdisciplinary fields.

An example of a micro diffusion apparatus in accordance with this invention for a single biological cell, for transporting materials across the cell membrane without the application of an electric field, is shown in FIG. 1. This components of this apparatus, from the bottom up, are an acrylic base 11, an intermediate silicon layer 12 (1 micron in thickness) with a portion 13 carved out to define the lateral boundaries of the lower of the two liquid chambers, a silicon nitride layer 14 serving as the barrier between the two chambers, a silicon washer 15 defining the lateral boundaries of the upper liquid chamber 16, and a glass cover plate 17. A hole 18 in the silicon nitride barrier serves as the opening, and a cell or contiguous cell mass such as tissue 19 is shown covering the hole. Channels extend through the acrylic base to serve as inlet and outlet channels for the liquids that pass through the upper and lower chambers, as shown by the arrows in the Figure.

When the pressure in the upper chamber 16 is higher than that in the lower chamber 13, the cell will be retained in position over the hole, serving as a plug separating the liquids in the two chambers from each other. When the composition of the solutions in the two chambers differs from that of the cell interior, mass transfer occurs across the cell membrane between the chambers and the cell. When the composition of the solution in one chamber differs from that in the other, mass transfer occurs through the cell from one chamber to the other. By precisely controlling the compositions of the solutions in the two chambers, one can precisely control the mass transfer rate and direction within the cell. Since the diameter of the opening 18 is known, one can precisely determine the mass transfer that occurs through the opening. The numerous applications of this microdiffusion device will be readily apparent.

For example, the device can be used to infuse a cell with a cryopreservative such as glycerol by filling the upper chamber 16 with physiological saline and the lower chamber 13 with glycerol. When using a cell 19 for which the mass transfer coefficient of glycerol across the cell membrane is known, one can readily calculate the amount of glycerol that will enter the cell and adjust the concentrations and exposure times to infuse the cell with the amount that is known to be required for cryopreservation.

An example of a microelectroporation apparatus in accordance with this invention for a single biological cell, is shown in FIG. 2. The apparatus is similar in construction to the microdiffusion apparatus of FIG. 1. Its structural components, from the bottom up, are an acrylic base 21, a lower silicon layer 22 with a portion carved out to define the lateral boundaries of the lower liquid chamber 23, a silicon nitride layer 24 (1 micron in thickness) serving as the barrier between the two chambers, an upper silicon layer 25 defining the lateral boundaries of the upper liquid chamber 26, and a cover consisting of an n+ poly-silicon layer (5,000 A in thickness) 27 and a silicon nitride layer (1 micron in thickness) 28. A hole 29 in the silicon nitride barrier 24 serves as the opening, and a cell 30 (or cell mass) covers the hole. Channels extend through the acrylic base to serve as inlets and outlets for the liquids that pass through the upper and lower chambers, as shown by the aπows in the Figure. A further layer of n+ poly-silicon (5,000 A) 31 resides above the acrylic base 21, and this layer, together with n+ poly-silicon layer 27 above the upper chamber 26 serve as the two electrodes. Each electrode is joined by electric leads to a pnnted circuit board 32 which controls the voltage applied between the electrodes and measures the current passmg between them

The microelectroporation apparatus shown m FIG 2 can be fabncated by conventional microfabncation techniques, typically involving chemical vapor deposition, maskmg, etching and sputtering The operation of the apparatus will be analogous to the operation of the microdiffusion apparatus of FIG 1 The movement of biological cells through the apparatus is achieved by suspendmg the cells m the liquid used to fill the upper chamber, and cells are drawn to the openmg, one at a time, by imposmg a pressure differential between the chambers, which also holds a cell m place once the cell has been drawn to the openmg A convement method of imposmg such a pressure differential is to mamtam atmosphenc pressure m the upper chamber while lowenng the pressure m the lower chamber below atmosphenc by attaching a synnge to the lower chamber and pulling on the syπnge plunger Care should be taken to limit the pressure differential to one that will not damage the cell

FIGS 3a and 3b illustrate to a different apparatus and method withm the scope of this mvention This apparatus and method involve a fluid suspension of biological cells flowmg through a conduit or flow channel, in which the cells pass through a region between a pair of electrodes The longitudinal cross section of FIG 3a shows the walls 41 of the channel, and a biological cell 42 passmg downward through the lumen of the channel (m the direction of the arrow) The transverse cross section of FIG 3b shows that the channel is rectangular m cross section, although other cross-sectional geometnes may be used Electrodes 43, 44 are formed as coatings on two opposmg walls of the channel The electrodes are connected through leads to a pnnted circuit board 45 which measures the impedance and controls the voltage applied to the electrodes The biological cell 42 is shown passmg through the region between the two electrodes The area of the cross section of the channel is large enough to permit the cell to pass through essentially unimpeded by the channel walls, and yet small enough that only one cell can pass through the mter-electrode region at a time In addition, each electrode 43, 44 is either approximately equal m length or slightly larger m length than the diameter of the biological cell so that the cell upon entering the region causes a significant or measurable decrease m the cuπent passmg through the region due to the voltage applied across electrodes The spacing of the electrodes, i e , the distance between them, is likewise subject to the same considerations The biological cells are suspended m a liquid solution of the species to be introduced mto the cells, and the suspension is passed through the channel A voltage is applied between the electrodes as suspension flows through the channel, and the cuπent between the electrodes (or the impedance) is monitored A significant drop m the cuπent mdicates the presence of a biological cell m the inter-electrode region Once the cell is detected m this manner, an electroporation pulse can be applied to the electrodes while the cell is still m the inter-electrode region, and impedance can be observed further to detect the onset of electroporation The species dissolved m the liquid solution will enter the cell as a result of the electroporation

Vanations on these structures and methods will be readily apparent to those skilled m the art For example, the barners descπbed above can be minimized or avoided by usmg microelectrodes that are the same size as or smaller than the biological cells Examples of such microelectrodes are carbon fiber microelectrodes (such as ProCFE, Axon Instruments, Foster City, California, USA) used m conjunction with high-graduation micromanipulators (such as those available from Naπshige MWH-3, Tokyo, Japan) Microelectrodes can be used m place of the electrodes shown m FIG 2 or in place of those shown m FIGS 3a and 3b

EXAMPLES The folio wing examples are put forth so as to provide those of ordinary skill m the art with a complete disclosure and descnption of how to make and use the present mvention, and are not mtended to limit the scope of what the mventors regard as their mvention nor are they mtended to represent that the expenments below are all or the only expenments performed Efforts have been made to ensure accuracy with respect to numbers used (e g amounts, temperature, etc ) but some expenmental eπors and deviations should be accounted for Unless mdicated otherwise, parts are parts by weight, molecular weight is weight average molecular weight, temperature is m degrees Centigrade, and pressure is at or near atmosphenc

EXAMPLE 1

A senes of expenments was performed usmg a microelectroporation system consisting of the microelectroporation device descπbed above and shown in FIG 2, combmed with flow and pressure control units and pressure gauges for the liquids to be circulated through the upper and lower chambers, a vanable DC power supply, a pulse generator and power amplifier for imposmg voltage pulses across the device, a digital oscilloscope for momtoπng the pulses, a fluorescent microscope, a CCD (charge coupled device) camera, and a computer with image processing and waveform processmg software Both chambers of the device were filled with physiological salme and cells were introduced mto the upper chamber Liquid motion in the top and bottom chambers was controlled by syringes The pressure m the upper chamber was atmosphenc while the pressure m the lower chamber was reduced below atmosphenc by pulling on the barrel of the syπnge connected to that chamber The voltage was applied m smgle square pulses ranging from zero to 120V m magnitude and from 2 microseconds to 100 milliseconds in duration The distance between the electrodes m the upper and lower chambers was 900 microns The tests in this example were performed usmg ND-1 human prostate adenocarcmoma cells with a typical diameter of 20 microns The openmg m the microelectroporation device was 5 microns in diameter A rectangular voltage pulse was applied with a duration of 60 milliseconds, and the pulse was applied at vaπous amplitudes ranging from 10V to 60V m mcrements of 5 volts With each pulse, the electnc current passmg through the openmg was measured Expenments were performed with the cells and were repeated both with the openmg stopped by a glass bead and with no obstruction at all in the opening The results in each case were expressed as microamperes of cuπent vs volts of pulse amplitude and are plotted m FIG 4, in which the upper curve (data pomts represented by x's) represents the unobstructed openmg, the lower curve (data pomts represented by astensks) represents the data taken with the glass bead residmg m the openmg, and the three middle curves (open squares, open upπght tnangles, and open inverted tnangles) represent data taken with three different ND-1 cells residmg m the openmg

The upper curve shows that the cuπent increases m a substantially steady manner as the voltage increases when there is no barner to the passage of current through the opemng The lower curve also shows a substantially steady nse as the voltage mcreases, although at a much lower level The current values shown m the lower curve represent stray currents through the device The curves of data taken with the ND-1 cells across the openmg show that at low voltages the cuπent is close m value to that obtamed when the openmg is closed by the glass bead while at high voltages the cuπent nses to the levels obtamed with an unobstructed opemng The transition is a sharp mcrease which is mdicative of the formation of pores m the cell membrane through which an electnc current can pass, i e , the onset of electroporation In all three cells, the transition occurred at voltages between 30V and 40V In two of the three cells (open squares and open upπght tnangles), the onset of electroporation occuπed essentially at the same voltage, while m the third (inverted tnangles), the onset occurred at a voltage that was lower than the other two by about 5 V This illustrates the value of controlling the process for individual cells to achieve optimal results

After the data shown m FIG 4 was generated, the pulses were reapphed m descending order of amplitude values, and the resultmg curves displayed hysteresis, i e , the curves obtamed with descendmg amplitudes were higher m voltage than those obtamed with ascending amplitudes. This indicated that the electroporation in these experiments was irreversible.

EXAMPLE 2

Using the same microelectroporation system used in Example 1, a series of tests were performed on rat hepatocytes (ATCC #CRL-1439), whose typical cell diameter was 20 microns, the microelectroporation apparatus having an opening that was 4 microns in diameter. Here as well, rectangular voltage pulses that were 60 milliseconds in duration were used, ranging in amplitude from 10V to 37.5V in increments of 5V in the portion from 10V to 30V and in increments of 2.5V in the portion from 30V to 37.5V. The experiments were performed in some cases only by increasing the amplitudes and in others by first increasing, then decreasing the amplitudes to evaluate reversibility. The results are plotted in the graphs shown in FIGS. 5a, 5b, 5c, and 5d. In each case, the upper curve (data points represented by circles) is the data taken with neither a cell nor a glass bead residing in the opening, the lower curve (data points represented by squares) is the data taken with a glass bead in the opening, and the middle curve (data points represented by triangles) is the data taken with a hepatocyte in the opening, using different hepatocytes for each of the four Figures.

In FIG. 5a, the amplitude was increased and not decreased, displaying an electroporation threshold voltage of between 25 V and 30V. In FIGS. 5b and 5c, the amplitude was first increased and then decreased to produce the two middle curves. Although the ascending and descending curves are not differentiated, they are substantially identical in each Figure, indicating that the cell membrane in each of these two cases resealed after each voltage pulse and thus that the pore formation was reversible. In the test represented by FIG. 5d, the cell disintegrated once the applied voltage exceeded 37.5V, although this is not shown in the Figure. It is significant to note that despite the fact that the same cell types were used in each of FIGS. 5a, 5b, 5c, and 5d, the electroporation threshold voltage differed among the individual cells, although all were within the range of 20V to 35V. Adaptation of the procedure to individual cells is readily achieved by monitoring the cuπent in this manner to note when the electroporation threshold occurs. Selection of the optimal exposure time, voltage, composition changes in the suπounding liquids, and other parameters of the system can then be made to achieve the desired treatment of the cell without destruction of the cell.

The methods described herein are useful tools in the laboratory for conducting fundamental research in the electroporation properties of biological cells, and useful tools in industry for processmg large quantities of cells in a flow-through manner By enabling one to observe and record the current flowmg through individual cells, one can control the amplitude and duration of the voltage pulse to achieve optimal results In addition, the devices descnbed and shown herem for use m practicmg the mvention can be constructed with transparent parts and of a size suitable for mounting on a microscope stage This will permit one to correlate the electncal current measurements to visual observations and fluorescence measurements mside the cell The device can be used to electπcally detect, through the measurement of cuπents, the pomt m time when a cell becomes lodged m the opemng as well as the pomt m time when pore formation is achieved m the cell membrane For larger scale and mdustnal applications, large numbers of microelectroporation devices of the type descnbed herem can be arranged in parallel For each cell, electπcal mformation mdicatmg the trapping of a cell in the openmg (such as a sharp drop m the current) can be used to generate a signal that will initiate an electroporation sequence, and further electπcal mformation mdicatmg the completion of electroporation (such as a sharp nse in current) will generate a signal that will release the cell (for example by eliminating or reversmg the pressure differential) and permit the next cell to flow toward the opemng

In addition to usmg the device and system of the mvention to move a mateπal into or out of the cell the system and device can be used m a diagnostic or analytic mode This is earned out by measunng electncal impedance of a cell or cells placed m a medium and usmg the measured electncal impedance information It is possible to deduce mformation relatmg to the mtegnty of cell membranes and thus provide for analysis It is also possible to compare the mformation to information previously obtamed on normal or diseased cells of the same type and thereby obtain diagnostic information For example, the electπcal impedance of a cell with an mtact membrane will be much high than the impedance of the same cell with impaired membrane Thus, analytically the process can provide mformation with respect to the structural mtegnty of the cell membrane Diagnostically the method can provide mformation with respect to the relative structural mtegnty of cell membranes

EXAMPLE 3 ELECTRICAL IMPEDANCE MAPPING OF ELECTROP ORATED DOMAINS

In order to illustrate the ability of EIT to monitor electroporation m tissue we have solved a mathematical simulation of the problem

To provide the necessary data for electroporation imagmg simulation, a simulated tissue phantom was created first using a 2-D fine-mesh FEM model (-1600 nodes, -3100 elements) The phantom, shown m FIG 9, consisted of a circular imagmg domam (20 mm radius, resistivity 500 ohm-cm for muscle with a vanable number of pomt source electrodes equally spaced around the peπphery Within this imagmg region, a smgle arbitranly shaped electroporated region was defined with a different resistivity An opposite electrode current injection pattern was used, providmg N(N-l)/2 independent voltage measurements where N is the number of electrodes The model was solved usmg the adaptive mesh generation and FEM solution algonthms available m MATLAB's Partial Differential Equation Toolbox (The Mathworks Inc ) An example mesh for the given geometry is shown m FIG 9 The mformation that the phantom module makes available to the reconstruction algoπthms represents data that would have been available duπng the electroporation part of an expeπment, 1 e cuπent and voltage at the different electrodes around the tissue From this data we attempted to reconstruct the ongmal image of the tissue that was mput m the model (It should be noted that a DC injection cuπent was used in place of the AC cuπent typical to EIT m order to simplify the problem The AC deπvation and implementation is a straightforward extension of that presented here ) A typical example for the voltage and current distnbution m the phantom during a simulated data acquisition step for an 8-electrode EIT system is illustrated m FIG 10

The data obtamed from the phantom was mput mto two EIT imagmg algonthms, one usmg the finite element method and the second the boundary element method to generate the impedance image The algoπthms use a standard Newton Raphson techmque to produce the image FIG 11 compares the image of a circular domam with two different electncal impedances m compaπson to the image of the ongmal phantom as recreated with the finite element technique and with the boundary element technique

Electncal impedance tomography can be used to image the electroporated region m tissue because EIT produces an image of the tissue from a map of the electncal impedance of the tissue and electroporation produces changes in impedance The electrodes for tissue electroporation imagmg may be different than those used for the electroporation process itself or may be the same

EXAMPLE 4 ELECTRICAL DETECTION OF CHANGE IN MEMBRANE PERMEABILITY

As part of our research on cell electroporation we have studied the electπcal characteπstics of cells during reversible and irreversible electroporation In reversible electroporation the cell is not damaged by the electroporation process and the membrane reseals In meversible electroporation the cell membrane is damaged and does not reseal In a set of experiments in which we have used ND-1 cells to measure currents through cells in the microelectroporation chip we have obtained results illustrated by FIGS. 8a and 8b. The results were obtained by exposing cells to triangular shaped electrical pulses (top curve) in 8a and 8b. The electrical currents flowing through the cells are shown in the bottom curve in 8a and 8b. FIG. 8a is for a cell that was iπeversible electroporated and FIG. 8b for a cell that was reversible electroporated. It can be easily noted that when the voltage was reduced in the reversible electroporated cell it retained the same values as during the voltage increase stage. However, in the irreversible case the current through the cell with the damaged membrane had a higher cuπent than in the intact cell. This leads to the conclusion that electrical currents flowing through cells can provide indication on changes in membrane permeability in general and a measure of the integrity of the cell membrane in particular under a variety of situations and not only during electroporation. For instance, cell viability is often measured with trypan blue or fluorescence dyes that penetrate through damaged membranes. These results show that an alternative method for detecting cells with damaged membranes would be to measure the electrical current-voltage relation across the cell. Similarly, there are compounds that induce pores in the cell membrane, such as ionophors. Measuring the current-voltage (impedance relation across a cell membrane could also detect if the membrane was impaired by these chemicals). Electrical measurements would have advantage over chemical means for detecting cell membrane damage because they would produce immediate information. A possible method for detecting changes in cell membrane permeability and in particular damaged cell membranes is to use the electroporation chip as described for the process of electroporation. The measure of damage would be the difference between an intact cell impedance and a damaged cell impedance as illustrated in FIGS. 8a and 8b . In tissue it would be possible to detect cells with damaged membranes in a similar way to the methods for detection of electroporation described here. While the present invention has been described with reference to the specific embodiments thereof, it should be understood by those skilled in the art that various changes may be made and equivalents may be substituted without departing from the true spirit and scope of the invention. In addition, many modifications may be made to adapt a particular situation, material, composition of matter, process, process step or steps, to the objective, spirit and scope of the present invention. All such modifications are intended to be within the scope of the claims appended hereto.

Claims

WHAT IS CLAIMED IS

1. A method, comprising the steps of: creating an electrical charge differential between a first point and a second point separated from the first point by an electrically conductive medium comprising a biological cell; measuring a first electrical parameter between the first and second points; and adjusting a second electrical parameter based on the measuring of the first electrical parameter.

2. The method of claim 1, wherein the first electrical parameter is selected from the group consisting of cuπent, voltage and electrical impedance and the second electrical parameter is selected from the group consisting of current, voltage and a combination of current and voltage.

3. The method of claim 1 further comprising: placing a material in the electrically conductive medium, and adjusting the second electrical parameter in order to move the material into the biological cell.

4. The method of claim 3, wherein the first point is a first electrode and the second point is a second electrode and the material is selected from the group consisting of a pharmaceutically active compound and a nucleotide sequence.

5. The method of claim 3 , wherein the measuring and adjusting are carried out at substantially continuously and at substantially the same time in a manner which causes a material in the medium to be moved into the biological cell and in a manner which allows for continued viability of the biological cell.

6. The method of claim 1, wherein the medium comprises a plurality

of biological cells.

7. The method of claim 6, wherein the biological cells comprise tissue present in a living organism.

8. The method of claim 7, wherein the living organism is an animal.

9. The method of claim 8, wherein the animal is selected from the group consisting of invertebrates and vertebrates.

10. The method of claim 9, wherein the vertebrate is a mammal.

11. The method of claim 10, wherein the mammal is a human.

12. A method, comprising the steps of: sending an electrical current between a first point and a second point separated from the first point by an electrically conductive medium comprising a biological cell; measuring a first electrical parameter in the medium; adjusting a second electrical parameter wherein the adjusting is carried out using information obtained from measuring the first electrical parameter.

13. The method of claim 12, wherein the first electrical parameter is selected from the group consisting of current, voltage and electrical impedance and the second electrical parameter is selected from the group consisting of current, voltage and a combination of current and voltage.

14. The method of claim 12, wherein the measuring and adjusting are carried out in a manner so as to cause electroporation of the cell without destroying a membrane of the cell.

15. The method of claim 12, further comprising: adding a therapeutically effective compound to the medium; and moving the compound into the cell.

16. The method of claim 14, further comprising: substantially blocking electrical current from between the first point and the second point except through the biological cell.

17. The method of claim 16, further comprising: placing a material in the electrically conductive medium, and adjusting the electrical cuπent in order to move the material into the biological cell.

18. A method for performing electroporation on a biological cell in a controlled manner, comprising:

(a) placing a biological cell in an electrically conductive medium and applying a voltage across the medium; (b) continuously detecting the ratio of electric cuπent through the medium to voltage across the medium; and

(c) adjusting the magnitude of the apphed voltage in accordance with changes in the detected cuπent-to-voltage ratio to achieve a controlled degree of electroporation of the biological cell.

19. A method in accordance with claim 18 in which step (b) comprises continuously detecting the current-to-voltage ratio as an indication of the electroporation of the biological cell, and step (c) comprises adjusting the duration of the applied voltage in accordance with the cuπent-to-voltage ratio to achieve a specific desired amount of electroporation.

20. A method in accordance with claim 18 wherein a plurality of the biological cells are placed in the electrically conductive medium, and the cuπent-to-voltage ratio is averaged over the plurality of biological cells, thereby achieving a controlled averaged degree of electroporation on the plurality of biological cells.

21. A method in accordance with claim 18 wherein the voltage is applied between two microelectrodes and the biological cell is positioned between the microelectrodes.

22. A method in accordance with claim 18 in which: the voltage is applied between two electrodes in a flow-through channel, the electrodes positioned to apply the voltage in a direction transverse to flow through the channel; step (a) comprises suspending the biological cell in the medium and continuously passing the medium through the channel; step (b) comprises further correlating the current-to-voltage ratio with the presence of the biological cell between the electrodes; and step (c) comprises adjusting the magnitude of the voltage while the biological cell is between the electrodes.

23. A method in accordance with claim 22 comprising suspending a plurality of the biological cells in the electrically conductive medium and continuously passing the medium through the channel such that approximately one cell at a time passes through the electrodes.

24. A method for performing electroporation in biological tissue in a controlled manner, comprising:

(a) placing the biological tissue in an electrically conductive medium and applying a voltage across the medium;

(b) continuously detecting the ratio of electric cuπent through the medium to voltage across the medium as an indication of the degree of electroporation in the biological tissue; and

(c) adjusting the magnitude of the applied voltage in accordance with changes in the magnitude of the cuπent-to-voltage ratio to achieve a controlled degree of electroporation in the biological tissue.

25. A method for the infusion of a biological cell with a chemical substance by electroporation in a manner that permits detection of the onset of and control of the electroporation, the method comprising:

(a) securing the biological cell in an electrical cell containing a liquid with the chemical substance dissolved therein, the electrical cell containing a barrier to electric current, the barrier aπanged such that, when a voltage is imposed across the electrical cell, the barrier restricts electric current flow to a flowpath passing through the biological cell while permitting substantially no electric current to bypass the biological cell;

(b) imposing a voltage across the electrical cell and monitoring the relative values of current passing through the cell and of the imposed voltage as an indication of the occuπence of electroporation in the cell.

26. A method in accordance with claim 25 in which the barrier divides first and second electrode chambers in the electrical cell and contains an opening smaller in width than the biological cell, and (a) comprises securing the biological cell over an opening such that the cell closes the opening.

27. A method in accordance with claim 26 in which the first electrode chamber contains a first electrically conducting liquid and the second electrode chamber contains a second electrically conducting liquid, and the chemical substance is dissolved in only one of the first and second electrically conducting liquids.

28 A method m accordance with claim 26 m which the first electrode chamber contams a first electncally conducting liquid and the second electrode chamber contams a second electπcally conducting liquid, and the chemical substance is dissolved m both of the first and second electπcally conducting liquids

29 A method m accordance with claim 26 in which (a) is accomplished by imposmg a pressure differential across the openmg to press the biological cell agamst one side of the openmg

30 A method m accordance with claim 26 m which (a) is accomplished by a coating on an area surrounding the opemng, the coatmg compnsed of a substance that binds to the barπer

31 A method m accordance with claim 26 m which the first electrode chamber is constructed and arranged to permit continuous flow of liquid therethrough, the method further compπsmg effecting continuous flow of a first electπcally conductmg liquid through the first electrode chamber

32 A method m accordance with claim 26 in which the first and second electrode chambers are constructed and arranged to permit continuous flow of liquid through each such chamber mdependently, the method further compπsmg effecting continuous flow of a first electπcally conducting liquid through the first electrode chamber and continuous flow of a second electπcally conducting liquid through the second electrode chamber

33 A method m accordance with claim 25 compπsmg securing a plurality of the biological cells m the electncal cell m which the bamer restncts cuπent flow to flowpaths passmg through all of the plurality of biological cells while permitting substantially no electnc current to bypass the plurality of biological cells

34 A method m accordance with claim 25 compπsmg securing only one the biological cell m the electπcal cell, and m which the bamer restncts cuπent flow to a flowpath through the only one biological cell while permitting substantially no electπc cuπent to bypass the only one biological cell

35 A method m accordance with claim 25 m which the electπc cell is transparent, and the method further compnses observing changes m the biological cell while the voltage is imposed

36. A method for the passage of a chemical species across a membrane of a biological cell in a controlled manner to achieve a selected rate of mass transfer across the membrane or to facilitate the determination of mass transfer properties of the membrane, the method comprising: (a) securing the cell over an opening in a barrier between first and second chambers, the opening being smaller in width than the cell such that the cell closes the opening, and

(b) placing a first liquid in the first chamber and a second liquid in the second chamber, at least one of the first and second liquids containing a solute at a concentration sufficiently higher than in the cell to cause the solute to diffuse into the cell.

37. A method in accordance with claim 36 in which securing the cell over the opening is accomplished by imposing a pressure differential across the opening to press the cell against one side of the opening.

38. A method in accordance with claim 36 in which securing the cell over the opening is accomplished by a coating on an area surrounding the opening, the coating comprised of a substance that binds to the membrane.

39. A method in accordance with claim 36 in which the first and second chambers are constructed and arranged to permit continuous flow of liquid through each such chamber independently, and (b) is accomphshed by continuous flow of the first hquid through the first chamber and continuous flow of the second liquid through the second chamber.

40. A method in accordance with claim 36 in which the concentration of the solute in the first liquid is sufficiently higher than in the second liquid to cause the solute to travel from the first liquid to the second liquid by diffusive transport, the barrier being sufficiently impermeable to the solute and the cell being sufficiently secured in the opening to restrict the diffusive transport to a diffusion path through the cell.

41. A method in accordance with claim 40 in which the solute is selected such that its mass transfer coefficient across the membrane is known, and the method is a method for infusing the cell with the solute and further comprises selecting the concentration of the solute in the first liquid and the period of time during which the diffusive transport is continued, both on the basis of the known mass transfer coefficient, to infuse the cell with a preselected amount of the solute. 42 A method m accordance with claim 40 further compπsmg monitoring changes in the cell while the solute is diffusing mto the cell, the changes bemg representative of the degree of infusion of the cell with the solute as a means of determining the rate of mass transfer of the solute across the membrane

43 A method m accordance with claim 36 m which the barner and the chambers are enclosed by a housmg that is transparent, the method further compnsmg observmg changes in the biological cell while the solute diffuses mto the biological cell

44 Apparatus for the infusion of a biological cell with a chemical substance by electroporation, the apparatus compnsmg an electnc cell containing an mtemal support to hold a biological cell and an mtemal barπer of a matenal substantially impermeable to electnc current, the barπer positioned to restrict electric current flow in the electπc cell to a flowpath crossmg the mtemal support and through any biological cell held thereby, and means for imposmg a voltage across the electnc cell and for momtonng the relative values of current and voltage as an indication of the occurrence and degree of electroporation m any biological cell held thereby

45 Apparatus m accordance with claim 44 in which the barπer divides the mteπor of the electπc cell mto first and second electrode chambers and the internal support is an opemng in the barner smaller in width than a biological cell

46 Apparatus in accordance with claim 44 further compπsmg means for imposmg a pressure differential across the openmg to lodge a biological cell in the openmg

47 Apparatus m accordance with claim 44 in which the first electrode chamber is a flow-through channel electncal current m order to move the matenal mto the biological cell