WO1996027787A1 - Membrane loader for gel electrophoresis - Google Patents

Membrane loader for gel electrophoresis Download PDF

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Publication number
WO1996027787A1
WO1996027787A1 PCT/US1996/002982 US9602982W WO9627787A1 WO 1996027787 A1 WO1996027787 A1 WO 1996027787A1 US 9602982 W US9602982 W US 9602982W WO 9627787 A1 WO9627787 A1 WO 9627787A1
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WO
WIPO (PCT)
Prior art keywords
sample
membrane
gel
buffer solution
loader
Prior art date
Application number
PCT/US1996/002982
Other languages
French (fr)
Inventor
Sallie Rice
Charles Browning
James Burke
Loi Nguyen
Original Assignee
Genetic Biosystems, Inc.
Priority date (The priority date is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the date listed.)
Filing date
Publication date
Application filed by Genetic Biosystems, Inc. filed Critical Genetic Biosystems, Inc.
Priority to AU54189/96A priority Critical patent/AU5418996A/en
Priority to EP96911246A priority patent/EP0871870A1/en
Publication of WO1996027787A1 publication Critical patent/WO1996027787A1/en

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Classifications

    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N27/00Investigating or analysing materials by the use of electric, electrochemical, or magnetic means
    • G01N27/26Investigating or analysing materials by the use of electric, electrochemical, or magnetic means by investigating electrochemical variables; by using electrolysis or electrophoresis
    • G01N27/416Systems
    • G01N27/447Systems using electrophoresis
    • G01N27/44704Details; Accessories
    • G01N27/44743Introducing samples

Definitions

  • This invention relates generally to the field of gel electrophoresis, and more particularly to an apparatus and method for loading samples into a gel of an electrophoretic gel system.
  • Electrophoresis gels are widely used in biotechnology for analyzing biomolecular sample materials such as proteins and nucleic acids. In molecular biology research laboratories, it is well known to use gel electrophoresis to separate and identify sample material based on size, charge and other aspects of the sample material. Biomolecules such as DNA, RNA and protein are commonly separated using this procedure. Electrophoresis involves the migration of electrically charged particles in a gel solution or suspension in the presence of an applied electric field. Samples are inserted or loaded into the gel of an electrophoretic gel system (EGS) and thereafter an electric field is applied to the gel. Each particle in the sample moves toward the electrode having an electrical polarity which is opposite the electrical polarity of the particle.
  • EGS electrophoretic gel system
  • the electrophoretic mobility of a sample particle is inversely proportional to the size of the particle.
  • Various species of a sample may be separated and identified due to differences in electrophoretic mobilities in the gel.
  • the gel also reduces the mixing, or "cross-talk", of various sample particles during the electrophoretic process. Gel electrophoresis thereby facilitates the stable separation and identification of sample material.
  • the initial step in manufacturing an EGS is "casting", or polymerization, of the gel.
  • a well-forming instrument such as a comb having teeth which extend downwardly toward a sample loading end of the EGS gel.
  • the comb teeth are inserted into the EGS gel before polymerization.
  • the comb is removed from the gel. thereby forming sample wells in the gel where the teeth were inserted.
  • a sample well-forming instrument is described in U.S. Patent No. 5,284,565 to Chu, et al.
  • the Chu comb forms sample wells in the EGS gel which taper downwardly toward the gel enclosure. Disadvantageously, it has proven difficult to form structurally consistent sample wells using these well-forming techniques.
  • FIGURES 1 -2 show a prior art electrophoretic gel system.
  • a gel 102 is disposed between two substantially rigid plates 104. 106 which are used to secure the gel 102 in place and to facilitate casting of the gel 102.
  • the gel 102 typically comprises agarose or polyacrylamide.
  • a well-forming comb 108 having a plurality of teeth or fingers 1 10 is used to form sample wells in the gel 102.
  • the comb 108 is inserted between the plates 104, 106 into an upper edge of the gel 102 before the gel polymerizes.
  • the comb 108 is removed from the upper edge of the gel 102.
  • a plurality of sample wells 1 12 are thus formed between the plates 104, 106 in the upper edge of the gel 102.
  • Liquid samples are then introduced into the sample wells 1 12 wherein they form individual sample pools, each separated by partitions 1 14 formed in the upper edge of the gel 102.
  • the apparatus 100 is immersed in an electrode buffer solution.
  • the buffer solution may be liquid, gel or paste.
  • the apparatus 100 is immersed in the electrode buffer solution so that the level of the solution 1 16 is slightly below the top edge of the plate 104.
  • an electric field is applied to the electrode buffer solution so that electric current passes through the buffer solution, sample material, and gel 102.
  • the samples in the sample wells 1 12 then migrate toward the bottom of the gel and separate due to their differing migration characteris ⁇ tics.
  • FIGURES 2a and 2b show a prior art horizontal EGS.
  • the horizontal EGS 200 includes a gel casting structure which has two substantially rigid removable dams 202 shaped to be received by the EGS 200.
  • the gel 204 is poured into the EGS 200 and is cast by the EGS walls and the removal dams 202.
  • the comb fingers 1 10 (FIGURES la and lb) are then inserted into the gel solution 204 before the gel congeals. After the gel congeals, the fingers 1 10 of the comb 108 are removed from the gel 204, as shown in FIGURE 2b.
  • the comb 108, and specifically the teeth 1 10, form sample wells 1 12 in the gel 204.
  • Sample material is then typically manually inserted into the wells 1 12 using a pipette.
  • One of the drawbacks of this sample insertion technique is that it requires a high degree of technical skill and dexterity. Consequently, the insertion of sample material into the wells is a time-intensive process which is prone to error and inadvertent spillage of sample material into the buffer solution. Therefore, there is a need for an improved gel electrophoresis method and apparatus which facilitates the loading of samples into an EGS.
  • the gel is immersed in an electrode buffer solution for electrophoretic separation. Similar to the apparatus of FIGURE 1 , the electrode buffer solution is filled to a level 1 16 which is sufficient to immerse the gel 204.
  • the EGS 200 typically includes connections to a power supply (not shown).
  • a cathode wire 206 is immersed in the electrode buffer solution at an upper end of the EGS 200 proximate the sample well end of the gel 204.
  • An anode wire 208 is immersed in the buffer solution at a bottom end of the EGS 200 near a distal end of the gel 204.
  • an electric field is typically applied to the buffer solution and the samples previously inserted into the sample wells 1 12 separate due to the electrophoretic effect.
  • Another drawback associated with the prior art EGS sample loading devices is due to the incomplete polymerization of certain types of gel material such as polyacrylamide due to the presence of a polymerization inhibitor. For example, due to the presence of oxygen, the area surrounding the comb teeth in prior art EGS loaders is often incompletely polymerized. Also, because the sample wells 1 12 are typically spaced in very close proximity to each other, the walls or partitions 114 are often quite fragile and as a result are easily damaged or destroyed. Another drawback associated with the prior art methods and apparatuses for loading samples into an EGS is the difficulty in removing undesirable materials such as urea from the sample wells after use.
  • the present invention provides such an apparatus and method.
  • the present invention is an apparatus and method for loading samples into a gel of an electrophoretic gel system (EGS).
  • the preferred sample loader includes a membrane which releasably retains the samples such that the samples are controllably released when the membrane is inserted into the gel of an EGS.
  • the sample loader includes a substrate having a membrane configured as a plurality of sample loading areas.
  • the sample loading areas are preferably diffusion-isolated from each other. Any practical means to isolate the diffusion of samples between the loading areas may be used.
  • the loading areas may be physically separated to prevent the diffusion of samples from one loading area to another.
  • sample inhibiting agents such as hydrophobic ink may be applied to the membrane to inhibit the diffusion of samples between the sample loading areas.
  • the substrate preferably comprises a strip-like material which is non-porous, non- conductive, relatively inert, neutrally charged, and inexpensive.
  • the substrate preferably comprises either celluloid or plastic.
  • the membrane preferably comprises either nylon or nitrocellulose.
  • the membrane is substantially thick and serves as its own substrate. Depending upon the samples to be loaded, the membrane may alternatively be neutrally, negatively or positively charged.
  • the sample loading areas preferably correspond to multiple columns of the EGS.
  • one or more samples to be subjected to electrophoretic action are applied to the sample loading areas of the membrane before the membrane is placed in contact with a previously polymerized gel. Cross-contamination of the samples is. in part, prevented by the physical spacing between each sample loading area.
  • the substrate is then positioned with respect to the EGS such that the sample loading areas are placed into contact with the polymerized gel immersed in buffer solution.
  • the membrane releasably binds the samples to the sample loading areas during insertion of the sample loading areas into the gel.
  • the membrane advantageously prevents contamination of electrode buffer solution and cross-talk or mixing between samples by inhibiting the diffusion of sample material into the gel or buffer solution before the membrane is activated by a release mechanism. Once the gel is activated by the release mechanism, the membrane releases substantially all of the samples into the gel where the samples are subjected to the electrophoretic separation and identification process.
  • the membrane of the present sample loader works with several different release mechanisms.
  • the membrane will release samples when the gel is activated via the application of an electric field to the buffer solution.
  • adding salt to change the salt concentration, adding acid or base to change the pH, heating or cooling, and strengthening or weakening the buffer solution are techniques that can be used to alter the releasing effect.
  • Other release mechanisms include the exposure of buffer solution to radiation, light, sonic waves, electromagnetic radiation, particle bombardment, and any other means that substantially causes the release of sample material from the membrane.
  • the present sample loader may alternatively be used alone or in conjunction with prior art EGS gels, loading apparatuses, and loading techniques.
  • the prior art well-forming combs may first be used to form sample wells in the prior art gels for electrophoresis. Thereafter, samples may be loaded into the gels by applying the samples to the membranes of the present sample loader, and inserting the sample loader into the sample wells.
  • the present sample loader may be used to form sample wells in the gel, and thereafter may be used to actively load samples in the wells by activating the gel with a release mechanism.
  • FIGURES la and lb are side perspective views of an electrophoresis apparatus used in the prior art electrophoretic gel systems (EGS).
  • FIGURES 2a and 2b are side perspective views of the electrophoresis apparatus of FIGURE 1 used in a prior art horizontal EGS.
  • FIGURES 3a and 3b are side perspective views of one preferred embodiment of the sample loader of the present invention intended for use in a vertical EGS.
  • FIGURE 4 is a side perspective view of a vertical EGS intended for use with the inventive sample loader of FIGURES 3a and 3b.
  • FIGURES 5a and 5b are side perspective views of prior art horizontal EGS system using the sample loader of FIGURES 3a and 3b.
  • FIGURE 6a is a front plan view of another preferred embodiment of the sample loader of the present invention.
  • FIGURE 6b is a side view of an alternative embodiment of the sample loader of the present invention.
  • FIGURE 6c is a front plan view of another preferred embodiment of the sample loader of the present invention.
  • FIGURE 7 is a front plan view of an end-loaded sample loader in accordance with the present invention.
  • FIGURE 8 is a front plan view of an alternative embodiment of the end-loaded sample loader of FIGURE 7.
  • FIGURES 3-4 show one preferred embodiment of the sample loader of the present invention intended for use in a vertical EGS.
  • FIGURES 5a and 5b show the sample loader of FIGURES 3-4 intended for use in a horizontal EGS.
  • the preferred sample loader 308 is shown before being placed in contact with an electrophoretic gel 102 which is disposed between two substantially rigid plates 104, 106 as described above with reference to FIGURES 1 and 2.
  • the sample loader 308 in one preferred embodiment, comprises a substrate 320 which has a plurality of sample loading fingers 310 formed in one side of the substrate 320. The fingers 310 extend downwardly away from a top edge 319 of the substrate 320.
  • the fingers 310 preferably include a loading area 312.
  • the loading areas correspond to the multiple columns of the EGS 200.
  • Each loading area 312 has an affixed membrane 306.
  • the sample loading areas 312 are "diffusion-isolated.” That is, cross- contamination of samples applied to each sample loading area is prevented in part by the physical spacing of the membranes 306 and fingers 310 or by some other convenient diffusion-isolation means.
  • the loader membrane 306 can have varying thicknesses and can thereby releasably retain more or less sample material. In an alternative embodiment, if the membrane 306 is sufficiently thick, it can serve as its own substrate.
  • the membranes 306 releasably retain or reversibly bind sample material to the loader 308. That is, the membranes 306 bind the sample material to the loader 308 when the sample is loaded or applied to the membranes 306 but actively release the sample material into the gel 102 upon activation of a release mechanism.
  • Various types of membrane material are described below in more detail with reference to FIGURE 6a.
  • Biomolecular samples 316 are quickly and easily applied by a technician to the loading areas 312 of the fingers 310.
  • the fingers 310 of the loader 308 are placed in contact with a proximal upper edge 314 of the gel 102 as shown in FIGURE 3b.
  • the fingers 310 are inserted far enough into the gel 102 so that the sample material 316 on the loading areas 312 does not contaminate the buffer solution after activation of the release mechanism. That is, the fingers 310 must be inserted far enough into the gel 102 so that the sample material 316 is inserted below the buffer solution level 1 16 and the edge 316 so that the sample material 316 does not diffuse into the buffer solution when released from the membranes 306.
  • the buffer solution may be liquid, gel, or paste.
  • the membranes 306 comprise materials which diffusion-isolate applied samples until the membranes 306 are activated by a release mechanism. That is, the membranes 306 preferably allow little or no diffusion of sample material 316 into the buffer solution or gel 102 until the gel 102. and the membranes 306, are activated by a release mechanism. However, upon the application of a releasing agent, the samples elute out of the membranes 306 and into the gel 102, where they are subjected to electrophoretic separation. In the preferred embodiment, the membrane 306 is selected to releasably bind a particular sample until the EGS electric field is applied to the buffer solution. Different membrane material may be used to diffusion- isolate different applied sample types, as discussed further below.
  • release mechanisms may be used in an EGS other than the application of an electric field to a buffer solution.
  • adding salt to change the salt concentration, adding acid or base to change the pH, heating or cooling the samples or the membrane, and/or strengthening or weakening the buffer solution can be used to alter the releasing effect.
  • the present sample loader can be used in an EGS which uses any of these releasing agents.
  • FIGURE 4 shows a vertical EGS 400 intended for use with the inventive sample loader 308 of FIGURES 3a and 3b.
  • the EGS 400 includes an upper cathode tank 402 and a lower anode tank 404. After the gel 102 polymerizes between the plates 104, 106, the plates 104, 106 are inserted vertically into the anode tank 404. Electrode buffer solution 408 is poured into the lower anode tank 404 and the upper cathode tank 402. A distal bottom edge of the polymerized gel 102 is thereby exposed to the electrode buffer solution 408 in the lower anode tank 404.
  • the upper edge 314 of the gel 102 is exposed to the electrode buffer solution 408 contained by the upper cathode tank 402 and the plate 104.
  • the electrode buffer solution 408 is filled in the upper cathode tank 402 to a level 1 16 which is below the top edge of the plate 104 yet which is sufficient to submerge the top edge 316 of the gel 102.
  • a cathode wire 410 is immersed in the buffer solution 408 and is preferably connected to a negative terminal of a DC power supply (not shown).
  • a anode wire 412 is similarly immersed into the electrode buffer solution 408 within the lower anode tank 404 and connected to the positive terminal of a DC power supply.
  • sample loader 308 After inserting the sample material using the sample loader 308 (FIGURES 3a and 3b) into the gel 102 as described above, samples are released out of the membrane and the electrophoretic separation process is triggered by activating the DC power supply and thereby applying an electric field to the gel 102.
  • the membranes 306 diffusion-isolate the sample material 316 and the sample material 316 thereby remains essentially bound to the membranes 306 unless and until the gel 102 is activated.
  • This diffusion-isolation or releasable retention of sample material to the membranes 306 reduces the potential for cross-talk between the different samples applied to the different fingers 310 and loading areas 312 of the loader 308. Furthermore, contamination of the electrode buffer solution 408 is prevented using the present loader 308.
  • the membranes 306 bind the sample material to the loader 308 and thereby prevent the inadvertent elution of sample material into the electrode buffer solution 408 when the sample material 316 is placed in contact with the gel 102.
  • the present sample loader 308 of FIGURES 3a and 3b and used in the vertical EGS 400 of FIGURE 4 facilitates the efficient, accurate, inexpensive, and rapid insertion of sample material into a gel for gel electrophoresis.
  • little technical skill or dexterity is required to load samples into an EGS using the present sample loader.
  • Samples can be quickly applied to the fingers 310 and more specifically the membranes 306 of the loader 308 before the loader 308 is placed in contact with the gel 102.
  • the loader 308 remains in contact with the gel 102 during the electrophoresis process, the structural integrity problems associated with the sample wells formed by the prior art sample loaders are eliminated.
  • the present sample loader 308 overcomes many of the drawbacks associated with the prior art sample loading devices and methods.
  • FIGURES 5a and 5b show the sample loader of FIGURES 3a and 3b intended for use in the horizontal EGS 200 described above with reference to FIGURES 2a and 2b.
  • the gel 204 is cast between two removable dams 202 before the insertion of sample material into the gel 204. After the gel 204 congeals, the dams 202 are removed from the device 200.
  • the device 200 is then filled with electrode buffer solution 408 to a level 1 16 which just exceeds an upper surface 220 of the gel 204.
  • sample material 316 is applied to the loading areas 312 and the membranes 306 of the sample loader 308 as described above with reference to FIGURES 3a and 3b.
  • the sample loader 308 is then positioned within the EGS 200 so that the loading areas 312 of the fingers 310 are positioned proximate a top edge 314 of the gel 204.
  • the sample material 316 contacts the gel 204 at the upper edge 314 as shown in FIGURE 5b.
  • the membranes 306 diffusion-isolate the sample material so that the sample material is reversibly bound to the membranes 306. Consequently, very little of the sample material diffuses into the gel 204 until the gel is activated by a release mechanism.
  • An electric field is then applied to the gel 204 via the cathode wire 206 and anode wire 208 as described above with reference to FIGURE 2b.
  • the biomolecular samples are then substantially released by the loader 308 and loaded into the gel 204.
  • FIGURE 6a shows details of a preferred embodiment of the sample loader of the present invention.
  • the sample loader 500 preferably comprises a substrate 502 and a plurality of fingers 504.
  • a lower portion of the substrate 502 includes a membrane 506 which diffusion-isolates applied sample material by reversibly binding the sample material to the fingers 504 of the sample loader 500.
  • the thickness of the membrane 506 may be varied to hold different sample amounts.
  • Sample loading areas 512 can be further defined in the fingers 504 by a plurality of sample inhibiting agents 514 which are formed through the membrane 506.
  • the sample inhibiting agent 514 may comprise hydrophobic ink which extends through each membrane 506 to the substrate 502 across the proximal end of each finger 504, as shown.
  • the hydrophobic ink 514 inhibits the migration or diffusion of sample material from one finger 504 to another.
  • the position of the ink 514 on each finger may also be used to define and control the size of the sample loading area of the membranes 506.
  • the hydrophobic ink 514 can be positioned within the membrane 506 in any configuration which inhibits the inadvertent diffusion of sample material from one finger 504 to another.
  • the hydrophobic ink 514' is vertically formed through the membrane 506 so that the ink 514' is equidistant between the fingers 504.
  • the membrane 506 preferably comprises material which diffusion-isolates or reversibly binds the biomolecular sample material before activation of a release mechanism, such as the application of an electric field. The material preferably binds and substantially retains the sample material to the loading area 512 when it is immersed in a standard electrophoretic buffer solution.
  • the membrane 506 when an electric field is applied to the buffer solution, the membrane 506 preferably releases a substantial portion of the bound sample material into the gel for separation and identification.
  • the sample transfer rate from the loading areas 512 to the gel is preferably substantially equivalent to the transfer rates between the sample wells and the gels in the prior art apparatuses.
  • the resolution of the sample bands produced using the present loader 500 and the resolution of the sample bands produced using the prior art apparatuses are also preferably substantially equivalent. Any membrane material which meets these requirements can be used to implement the membrane of the present invention. However, a number of factors can affect the performance and therefore the selection of membrane material.
  • the sample type can affect the membrane's ability to releasably bind and retain the sample.
  • DNA molecules appear to be more easily bound and retained by the membranes investigated than are RNA molecules.
  • proteins are less effectively bound and retained by the membranes than are DNA molecules.
  • the RNA samples generally are released into the gel solution upon activation just as effectively as are the DNA samples.
  • the membrane's performance can vary under varying conditions of buffer solution pH, temperature, salt concentration, and strength. These varying conditions can affect the amount of electric charge required to fully release the samples from the membrane 506.
  • pre-wetting, pre-spotting. and drying time for pre-treated membranes can also affect membrane performance.
  • the membrane 506 shown in FIGURE 6a preferably is used to load any type of biomolecular sample into an electrophoretic gel under typical laboratory conditions.
  • the membrane preferably comprises either nitrocellulose or nylon.
  • the nylons may either be electrically neutral, or positively or negatively charged.
  • the samples preferably loaded by the present sample loader 500 are double-stranded DNA (dsDNA), single-stranded DNA (ssDNA), RNA, and proteins.
  • the composition of the membrane 506 depends upon the samples to be loaded by the present sample loader.
  • the membrane 506 preferably comprises either neutral nylon or nitrocellulose.
  • neutral nylons include Biotrans® available from ICN. located in Costa Mesa, CA., and Immobilon-S® available from Millipore, located in Bedford, MA.
  • nitrocellulose materials include BA85 available from Schleicher & Schuell, located in Keene, NH, and Bioblot-NC® available from Costar, located in Cambridge, MA.
  • nitrocellulose membranes are preferred when performing electrophore ⁇ sis of ssDNA and sequencing reactions.
  • the membrane 506 preferably comprises Teflon® or polyvinylidene fluoride (PVDF) nylon.
  • the present invention contemplates the use of any membrane which adequately releasably binds and retains sample material before activation of a release mechanism, yet which efficiently releases a substantial portion of the sample material into the gel after the system is activated by a release mechanism.
  • the present sample loader 500 preferably includes a substrate 502 which structurally supports the membrane 506.
  • the substrate 502 preferably comprises a non-conductive, relatively inert, non-porous, neutrally charged, inexpensive material.
  • the substrate preferably comprises either celluloid or plastic.
  • the substrate 502 may be manufactured using a number of techniques. For example, the substrate 502 may first be cut to a desired width. The fingers 504 may then be formed in one side of the substrate 502 by cutting, scoring or punching away areas 520 between the fingers 504. Preferably, the fingers 504 are formed sufficiently long to prevent capillary action or wicking of buffer solution from contaminating the samples applied to the membrane loading areas. Similarly, the fingers 504 are preferably sufficiently long to prevent wicking of a sample from a first loading area 512 to a second loading area 512 on another finger 504.
  • the present sample loader 500 is manufactured by placing the substrate 502 (which is typically formed into strips) into a membrane slurry material.
  • the membrane slurry is placed in contact with the substrate 502 until it solidifies upon the surface of the substrate.
  • the fingers 504 are formed in the substrate by punching or cutting away areas between the fingers.
  • Sample loading areas 512 are defined in the fingers 504 by scoring substantially horizontal lines across approximate midpoints of the fingers 504. During the scoring process, the solidified membrane material is cut away from the substrate 502.
  • the substrate 502 is left in tact.
  • the scored membrane is filled with hydrophobic ink 514 as shown in FIGURE 6a and described above.
  • Other alternative embodiments use photoetching or photomasking techniques to define the sample loading areas 512.
  • the membrane 506 may be formed on the finger side of the substrate 502 by any convenient method, such as screening liquid membrane material to the substrate 502 or dipping the substrate 502 into a liquid membrane pool for a time which is sufficient to allow the membrane material to adhere to the substrate 502.
  • the membrane may be formed by cutting membrane bulk material into strips of equal widths and affixing the strips on the substrate 502 as shown in FIGURE 6a. That is, the strips of membrane can be used to define the fingers 504 of the sample loader 500.
  • the membrane comprises sheets of plastic-backed nitrocellulose material available from Schleicher & Schuell. As described above with reference to FIGURE 3a, one alternative embodiment of the sample loader 500 shown in FIGURE 6a eliminates the necessity for the substrate 502.
  • the membrane 506 comprises material which is sufficiently rigid, and if the membrane 506 is sufficiently thick, the entire substrate 502 can be replaced with membrane material (i.e., the membrane 506 is used as the substrate).
  • the fingers 504, sample loading areas 512, and sample inhibiting agents 514 (if necessary) are formed into the membrane as described above with reference to the preferred embodiment.
  • the substrate 502 is substantially thicker than the substrate of the preferred embodiment and the membrane 506.
  • the relatively thin membrane 506 and fingers 504 are attached as "legs" to the bottom 503 of the substrate 502.
  • FIGURE 6c shows a front plan view of yet another alternative embodiment of the present invention.
  • the embodiment of FIGURE 6c is similar to that shown in FIGURE 6a with the exception that the fingers 504 have been replaced by "virtual fingers" which are formed into the substrate 502'.
  • the sample loader 500' shown in FIGURE 6c is preferably manufactured by screening membrane material 506' onto a sample loading portion of the substrate 502' and thereby creating sample loading areas 512' (or "virtual fingers") onto the substrate 502'. As described above with reference to FIGURE 6a. the sample loading areas 512' diffusion-isolate sample material which is applied thereto until the membrane 506' is activated by a release mechanism.
  • the notches 520 of FIGURE 6a are replaced by the virtual notches 520' which are merely areas of diffusion-isolation between the sample loading areas 512'.
  • the embodiment shown in FIGURE 6c is useful in EGS applications which do not require sample loading fingers which extend downwardly toward the EGS gel.
  • the alternative embodiment shown in FIGURE 6c can alternatively be manufactured by first applying or affixing membrane material to the sample loading portion of the substrate 502'. and then scoring the membrane 506' to create the virtual notches 520' (i.e., areas where membrane material is removed from the substrate 502') as shown in FIGURE 6c.
  • the sample loading areas 512' can be diffusion-isolated from each other using a chemical isolation means such as the hydrophobic ink described above with reference to FIGURE 6a. If hydrophobic ink is used, the loading areas 512' can be formed by first deeply scoring into the membrane 502' and thereafter filling the scored portions of the substrate with the ink.
  • FIGURE 7 shows an end-loaded sample loader 600. Similar to the sample loader of FIGURE 6a. the end-loaded sample loader 600 preferably includes a substrate 502, a plurality of teeth or sample loading fingers 504, each having a proximal end 602 and a distal end 604, wherein the fingers extend downwardly away from the proximal end 602, a sample loading area 512 at the distal end 604 of the fingers 504, and a membrane 606.
  • the membrane 606 is affixed to the distal end 604 of the fingers 504 so that only a very small percentage of the total finger length is covered by the membrane 606.
  • the membrane 506 of the sample loader 500 of FIGURES 6a and 6b covers a substantial length of the fingers.
  • sample material is applied to the sample loading areas 512 by simply dipping or otherwise adhering the sample material to the membranes 606.
  • the membrane 606 should be sufficient to hold a sample in solution where the drop volume is at least approximately 0.3 ⁇ L.
  • the loader does not require use of a sample inhibiting agent such as the hydrophobic ink described above with reference to the preferred embodiment shown in FIGURE 6. Because a sample is applied only to the distal end 604 of a finger 504, and not along the entire length of the finger, the sample is less likely to diffuse from one finger to either the buffer solution or another finger.
  • a sample inhibiting agent such as the hydrophobic ink described above with reference to the preferred embodiment shown in FIGURE 6.
  • an alternative end-loaded sample loader might include such a sample inhibiting agent similar to that described above with reference to FIGURE 6.
  • the sample inhibiting agent preferably comprises hydrophobic ink which inhibits the migration or diffusion of sample material from one finger 604 to another.
  • the ink is preferably positioned across the width of each finger 504 at the proximal ends 602 of the fingers 504.
  • the membrane 606 can alternatively serve as its own substrate.
  • FIGURE 8 shows another alternative embodiment of the end-loaded sample loader of FIGURE 7. Similar to the loader of FIGURE 7, the sample loader shown in FIGURE 8 preferably includes a substrate 502, and a plurality of sample loading fingers 504, each having a proximal end 702 and a distal end 704, wherein the fingers 504 extend downwardly away from the proximal end 702.
  • the fingers 504 include a three- dimensional sample loading area 712 which surrounds the distal end 704 of the fingers 504.
  • the sample loading areas 712 are preferably formed by dipping the fingers 504 into a pool of membrane material, removing the loader 700 from the pool of membrane material, and allowing the membranes to solidify into the colloidons shown in FIGURE 8.
  • the loading areas 712 are much more three-dimensional than the rectangularly-shaped loading areas 512 of the sample loader shown in FIGURE 7 (the loading areas 512 are substantially two-dimensional), the loading areas 712 accommodate a greater volume of sample material than do the loading areas 512.
  • samples are typically applied to the membranes covering the sample loading areas 712 and allowed to dry. Similar to the sample loader of FIGURE 7. if the fingers 504 are sufficiently long, a sample inhibiting agent need not be used. Because samples are applied only to the sample loading areas 712, the samples are less likely to diffuse from one finger to another and thereby cause cross-contamination of samples.
  • an alternative end-loaded sample loader might include sample inhibiting agents similar to those described above with reference to FIGURES 6a and 6b.
  • All of the embodiments of the present invention of an apparatus and method of loading samples into a gel of an EGS may also be used with the prior art systems which first form sample wells in the gels and then load the wells with the samples to be tested.
  • the present invention may be used to load sample material into the sample wells after the gel polymerizes.
  • the present invention may be used to load samples into sample wells previously formed by a prior art well-forming device.
  • the present invention is a sample loader for an EGS having well- defined diffusion-isolated sample loading areas.
  • the sample loading areas preferably include a membrane which releasably retains applied sample material until and unless the membrane is activated by a release mechanism.
  • the sample material When immersed in a buffer solution and/or gel of an EGS, the sample material sufficiently adheres to the membrane so that the sample material does not diffuse substantially into the gel before activation of a release mechanism. However, when activated by a release mechanism, the membrane releases a substantial portion of the sample material into the gel and allows the sample material to undergo an electrophoretic process.
  • a number of different means may be used to diffusion-isolate the loading areas.
  • the loading areas may be chemically-isolated using a hydrophobic ink.
  • the substrate of the loader may be scored thereby forming "virtual fingers" in the substrate.
  • Hydrophobic ink may alternatively be used to fill in the scored areas and thus further diffusion-isolate the virtual fingers.
  • the side of the sample holder which is grasped by a technician may be circularly-shaped, or may include a handle for easy handling.
  • the width of the fingers and membranes can also be varied depending upon the amount of sample material to be loaded.
  • the loader can be manufactured by arranging parallel sheets of substrate under a single membrane sheet, and adhering the membrane to both sides of the substrates. Each parallel sheet thereby forms a finger of the sample loader.
  • the method of using the present sample loader discloses placing the sample loading areas into contact with the electrophoretic gel material, the present sample loader can also be used by inserting the sample loading areas and fingers into the gel.

Abstract

An apparatus for loading sample onto an electrophoretic gel comprising a membrane which releasably retains samples such that the samples are actively released when the membrane is placed in contact with the gel. In one embodiment the sample loader (308) comprises a substrate (320) which has a plurality of sample loading fingers (310) which extend downwardly away from the top edge (319). The sample loading fingers (310) preferably include loading areas (312). Each loading area (312) has an affixed membrane (306).

Description

MEMBRANE LOADER FOR GEL ELECTROPHORESIS
BACKGROUND OF THE INVENTION
1. Field of the Invention
This invention relates generally to the field of gel electrophoresis, and more particularly to an apparatus and method for loading samples into a gel of an electrophoretic gel system.
2. Description of Related A rt
Electrophoresis gels are widely used in biotechnology for analyzing biomolecular sample materials such as proteins and nucleic acids. In molecular biology research laboratories, it is well known to use gel electrophoresis to separate and identify sample material based on size, charge and other aspects of the sample material. Biomolecules such as DNA, RNA and protein are commonly separated using this procedure. Electrophoresis involves the migration of electrically charged particles in a gel solution or suspension in the presence of an applied electric field. Samples are inserted or loaded into the gel of an electrophoretic gel system (EGS) and thereafter an electric field is applied to the gel. Each particle in the sample moves toward the electrode having an electrical polarity which is opposite the electrical polarity of the particle. The electrophoretic mobility of a sample particle is inversely proportional to the size of the particle. Various species of a sample may be separated and identified due to differences in electrophoretic mobilities in the gel. The gel also reduces the mixing, or "cross-talk", of various sample particles during the electrophoretic process. Gel electrophoresis thereby facilitates the stable separation and identification of sample material.
Typically, the initial step in manufacturing an EGS is "casting", or polymerization, of the gel. Common techniques used to cast the gel employ a well-forming instrument such as a comb having teeth which extend downwardly toward a sample loading end of the EGS gel. In these systems, the comb teeth are inserted into the EGS gel before polymerization. After the gel polymerizes, the comb is removed from the gel. thereby forming sample wells in the gel where the teeth were inserted. One example of such a sample well-forming instrument is described in U.S. Patent No. 5,284,565 to Chu, et al. The Chu comb forms sample wells in the EGS gel which taper downwardly toward the gel enclosure. Disadvantageously, it has proven difficult to form structurally consistent sample wells using these well-forming techniques.
FIGURES 1 -2 show a prior art electrophoretic gel system. As shown in the electrophoresis apparatus 100 of FIGURE la, a gel 102 is disposed between two substantially rigid plates 104. 106 which are used to secure the gel 102 in place and to facilitate casting of the gel 102. The gel 102 typically comprises agarose or polyacrylamide. A well-forming comb 108 having a plurality of teeth or fingers 1 10 is used to form sample wells in the gel 102. As shown in FIGURE la, the comb 108 is inserted between the plates 104, 106 into an upper edge of the gel 102 before the gel polymerizes. As shown in FIGURE lb, after the gel polymerizes, the comb 108 is removed from the upper edge of the gel 102. A plurality of sample wells 1 12 are thus formed between the plates 104, 106 in the upper edge of the gel 102. Liquid samples are then introduced into the sample wells 1 12 wherein they form individual sample pools, each separated by partitions 1 14 formed in the upper edge of the gel 102. To facilitate the electrophoresis process, the apparatus 100 is immersed in an electrode buffer solution. The buffer solution may be liquid, gel or paste. As shown in FIGURE 1 b, the apparatus 100 is immersed in the electrode buffer solution so that the level of the solution 1 16 is slightly below the top edge of the plate 104. After the liquid samples are introduced into the sample wells 1 12, an electric field is applied to the electrode buffer solution so that electric current passes through the buffer solution, sample material, and gel 102. The samples in the sample wells 1 12 then migrate toward the bottom of the gel and separate due to their differing migration characteris¬ tics.
FIGURES 2a and 2b show a prior art horizontal EGS. The horizontal EGS 200 includes a gel casting structure which has two substantially rigid removable dams 202 shaped to be received by the EGS 200. Before solidification or congelation of a gel 204, the gel 204 is poured into the EGS 200 and is cast by the EGS walls and the removal dams 202. The comb fingers 1 10 (FIGURES la and lb) are then inserted into the gel solution 204 before the gel congeals. After the gel congeals, the fingers 1 10 of the comb 108 are removed from the gel 204, as shown in FIGURE 2b. The comb 108, and specifically the teeth 1 10, form sample wells 1 12 in the gel 204. Sample material is then typically manually inserted into the wells 1 12 using a pipette. One of the drawbacks of this sample insertion technique is that it requires a high degree of technical skill and dexterity. Consequently, the insertion of sample material into the wells is a time-intensive process which is prone to error and inadvertent spillage of sample material into the buffer solution. Therefore, there is a need for an improved gel electrophoresis method and apparatus which facilitates the loading of samples into an EGS.
As shown in FIGURE 2b, the gel is immersed in an electrode buffer solution for electrophoretic separation. Similar to the apparatus of FIGURE 1 , the electrode buffer solution is filled to a level 1 16 which is sufficient to immerse the gel 204. The EGS 200 typically includes connections to a power supply (not shown). As shown in FIGURE 2b, a cathode wire 206 is immersed in the electrode buffer solution at an upper end of the EGS 200 proximate the sample well end of the gel 204. An anode wire 208 is immersed in the buffer solution at a bottom end of the EGS 200 near a distal end of the gel 204. Thereafter, as described above, an electric field is typically applied to the buffer solution and the samples previously inserted into the sample wells 1 12 separate due to the electrophoretic effect.
Another prior art gel electrophoresis system and sample loader is disclosed in U.S. Patent No. 5,275,710 issued to Gombocz et al. Gombocz teaches a sample loader or applicator which has a plurality of applicator channels covered by an absorbent material (such as a wick) which prevents the uninhibited flow of sample material into the gel. When the wicks are loaded with a measured amount of sample material, the applicator is lowered into the gel so that the wicks contact the gel, which allows the sample material to perfuse through the wicking material and into the gel. Disadvanta- geously, the applicator taught by Gombocz allows sample material to diffuse into the gel and surrounding buffer before the gel is activated by applying an electric field. Therefore, a need exists for a sample loading apparatus and method for loading samples into an EGS which allows samples to be easily, quickly and accurately loaded into the gel yet which inhibits the electrophoretic separation of the samples until activation by the release mechanism.
One of the problems associated with the prior art sample loading apparatuses is the potential for inadvertent cross-contamination via the buffer solution. As shown in FIGURE lb, if the samples overflow the sample wells 1 12, the buffer solution becomes contaminated with sample material, which may lead to erroneous results due to mixing of sample material between sample wells. Therefore, there is a need for a method and apparatus for loading sample material into an EGS which inhibits the diffusion of sample material into the gel or buffer before electrophoretic action commences.
Another drawback associated with the prior art EGS sample loading devices is due to the incomplete polymerization of certain types of gel material such as polyacrylamide due to the presence of a polymerization inhibitor. For example, due to the presence of oxygen, the area surrounding the comb teeth in prior art EGS loaders is often incompletely polymerized. Also, because the sample wells 1 12 are typically spaced in very close proximity to each other, the walls or partitions 114 are often quite fragile and as a result are easily damaged or destroyed. Another drawback associated with the prior art methods and apparatuses for loading samples into an EGS is the difficulty in removing undesirable materials such as urea from the sample wells after use.
Therefore, there is a need for an improved apparatus and method for loading sample material into a gel of an EGS. The present invention provides such an apparatus and method.
SUMMARY OF THE INVENTION The present invention is an apparatus and method for loading samples into a gel of an electrophoretic gel system (EGS). The preferred sample loader includes a membrane which releasably retains the samples such that the samples are controllably released when the membrane is inserted into the gel of an EGS. In one preferred embodiment, the sample loader includes a substrate having a membrane configured as a plurality of sample loading areas. The sample loading areas are preferably diffusion-isolated from each other. Any practical means to isolate the diffusion of samples between the loading areas may be used. For example, the loading areas may be physically separated to prevent the diffusion of samples from one loading area to another. Alternatively, sample inhibiting agents such as hydrophobic ink may be applied to the membrane to inhibit the diffusion of samples between the sample loading areas.
The substrate preferably comprises a strip-like material which is non-porous, non- conductive, relatively inert, neutrally charged, and inexpensive. For example, the substrate preferably comprises either celluloid or plastic. The membrane preferably comprises either nylon or nitrocellulose. In an alternative embodiment, the membrane is substantially thick and serves as its own substrate. Depending upon the samples to be loaded, the membrane may alternatively be neutrally, negatively or positively charged.
The sample loading areas preferably correspond to multiple columns of the EGS. In use, one or more samples to be subjected to electrophoretic action are applied to the sample loading areas of the membrane before the membrane is placed in contact with a previously polymerized gel. Cross-contamination of the samples is. in part, prevented by the physical spacing between each sample loading area. The substrate is then positioned with respect to the EGS such that the sample loading areas are placed into contact with the polymerized gel immersed in buffer solution. The membrane releasably binds the samples to the sample loading areas during insertion of the sample loading areas into the gel.
The membrane advantageously prevents contamination of electrode buffer solution and cross-talk or mixing between samples by inhibiting the diffusion of sample material into the gel or buffer solution before the membrane is activated by a release mechanism. Once the gel is activated by the release mechanism, the membrane releases substantially all of the samples into the gel where the samples are subjected to the electrophoretic separation and identification process.
The membrane of the present sample loader works with several different release mechanisms. For example, the membrane will release samples when the gel is activated via the application of an electric field to the buffer solution. Also, adding salt to change the salt concentration, adding acid or base to change the pH, heating or cooling, and strengthening or weakening the buffer solution, are techniques that can be used to alter the releasing effect. Other release mechanisms include the exposure of buffer solution to radiation, light, sonic waves, electromagnetic radiation, particle bombardment, and any other means that substantially causes the release of sample material from the membrane.
The present sample loader may alternatively be used alone or in conjunction with prior art EGS gels, loading apparatuses, and loading techniques. For example, the prior art well-forming combs may first be used to form sample wells in the prior art gels for electrophoresis. Thereafter, samples may be loaded into the gels by applying the samples to the membranes of the present sample loader, and inserting the sample loader into the sample wells. Alternatively, the present sample loader may be used to form sample wells in the gel, and thereafter may be used to actively load samples in the wells by activating the gel with a release mechanism.
The details of the preferred embodiment of the present invention are set forth in the accompanying drawings and the description below. Once the details of the invention are known, numerous additional innovations and changes will become obvious to one skilled in the art.
BRIEF DESCRIPTION OF THE DRAWINGS FIGURES la and lb are side perspective views of an electrophoresis apparatus used in the prior art electrophoretic gel systems (EGS).
FIGURES 2a and 2b are side perspective views of the electrophoresis apparatus of FIGURE 1 used in a prior art horizontal EGS.
FIGURES 3a and 3b are side perspective views of one preferred embodiment of the sample loader of the present invention intended for use in a vertical EGS.
FIGURE 4 is a side perspective view of a vertical EGS intended for use with the inventive sample loader of FIGURES 3a and 3b.
FIGURES 5a and 5b are side perspective views of prior art horizontal EGS system using the sample loader of FIGURES 3a and 3b.
FIGURE 6a is a front plan view of another preferred embodiment of the sample loader of the present invention.
FIGURE 6b is a side view of an alternative embodiment of the sample loader of the present invention.
FIGURE 6c is a front plan view of another preferred embodiment of the sample loader of the present invention.
FIGURE 7 is a front plan view of an end-loaded sample loader in accordance with the present invention.
FIGURE 8 is a front plan view of an alternative embodiment of the end-loaded sample loader of FIGURE 7.
Like reference numbers and designations in the various drawings refer to like elements. DETAILED DESCRIPTION OF THE INVENTION
Throughout this description, the preferred embodiment and examples shown should be considered as exemplars, rather than as limitations on the present invention.
FIGURES 3-4 show one preferred embodiment of the sample loader of the present invention intended for use in a vertical EGS. FIGURES 5a and 5b show the sample loader of FIGURES 3-4 intended for use in a horizontal EGS. Referring now to FIGURE 3a, the preferred sample loader 308 is shown before being placed in contact with an electrophoretic gel 102 which is disposed between two substantially rigid plates 104, 106 as described above with reference to FIGURES 1 and 2. As described below in more detail with reference to FIGURE 6a, the sample loader 308, in one preferred embodiment, comprises a substrate 320 which has a plurality of sample loading fingers 310 formed in one side of the substrate 320. The fingers 310 extend downwardly away from a top edge 319 of the substrate 320. The fingers 310 preferably include a loading area 312. The loading areas correspond to the multiple columns of the EGS 200. Each loading area 312 has an affixed membrane 306. In use, one or more samples to be subjected to electrophoretic action are placed on the individual membranes 306. As described below in more detail with reference to FIGURE 6a. the sample loading areas 312 are "diffusion-isolated." That is, cross- contamination of samples applied to each sample loading area is prevented in part by the physical spacing of the membranes 306 and fingers 310 or by some other convenient diffusion-isolation means.
The loader membrane 306 can have varying thicknesses and can thereby releasably retain more or less sample material. In an alternative embodiment, if the membrane 306 is sufficiently thick, it can serve as its own substrate.
The membranes 306 releasably retain or reversibly bind sample material to the loader 308. That is, the membranes 306 bind the sample material to the loader 308 when the sample is loaded or applied to the membranes 306 but actively release the sample material into the gel 102 upon activation of a release mechanism. Various types of membrane material are described below in more detail with reference to FIGURE 6a.
Biomolecular samples 316 are quickly and easily applied by a technician to the loading areas 312 of the fingers 310. The fingers 310 of the loader 308 are placed in contact with a proximal upper edge 314 of the gel 102 as shown in FIGURE 3b. The fingers 310 are inserted far enough into the gel 102 so that the sample material 316 on the loading areas 312 does not contaminate the buffer solution after activation of the release mechanism. That is, the fingers 310 must be inserted far enough into the gel 102 so that the sample material 316 is inserted below the buffer solution level 1 16 and the edge 316 so that the sample material 316 does not diffuse into the buffer solution when released from the membranes 306. Similar to the prior art EGSs described above, the buffer solution may be liquid, gel, or paste.
After the sample is loaded onto the gel 102, but before activation of the release mechanism, the sample material 316 remains releasably bound to the membranes 306 of the loader 308. The membranes 306 comprise materials which diffusion-isolate applied samples until the membranes 306 are activated by a release mechanism. That is, the membranes 306 preferably allow little or no diffusion of sample material 316 into the buffer solution or gel 102 until the gel 102. and the membranes 306, are activated by a release mechanism. However, upon the application of a releasing agent, the samples elute out of the membranes 306 and into the gel 102, where they are subjected to electrophoretic separation. In the preferred embodiment, the membrane 306 is selected to releasably bind a particular sample until the EGS electric field is applied to the buffer solution. Different membrane material may be used to diffusion- isolate different applied sample types, as discussed further below.
Many different release mechanisms may be used in an EGS other than the application of an electric field to a buffer solution. For example, adding salt to change the salt concentration, adding acid or base to change the pH, heating or cooling the samples or the membrane, and/or strengthening or weakening the buffer solution can be used to alter the releasing effect. The present sample loader can be used in an EGS which uses any of these releasing agents.
FIGURE 4 shows a vertical EGS 400 intended for use with the inventive sample loader 308 of FIGURES 3a and 3b. The EGS 400 includes an upper cathode tank 402 and a lower anode tank 404. After the gel 102 polymerizes between the plates 104, 106, the plates 104, 106 are inserted vertically into the anode tank 404. Electrode buffer solution 408 is poured into the lower anode tank 404 and the upper cathode tank 402. A distal bottom edge of the polymerized gel 102 is thereby exposed to the electrode buffer solution 408 in the lower anode tank 404. The upper edge 314 of the gel 102 is exposed to the electrode buffer solution 408 contained by the upper cathode tank 402 and the plate 104. As described above with reference to FIGURES lb, 2b, and 3b, the electrode buffer solution 408 is filled in the upper cathode tank 402 to a level 1 16 which is below the top edge of the plate 104 yet which is sufficient to submerge the top edge 316 of the gel 102.
A cathode wire 410 is immersed in the buffer solution 408 and is preferably connected to a negative terminal of a DC power supply (not shown). A anode wire 412 is similarly immersed into the electrode buffer solution 408 within the lower anode tank 404 and connected to the positive terminal of a DC power supply.
After inserting the sample material using the sample loader 308 (FIGURES 3a and 3b) into the gel 102 as described above, samples are released out of the membrane and the electrophoretic separation process is triggered by activating the DC power supply and thereby applying an electric field to the gel 102. Advantageously, the membranes 306 diffusion-isolate the sample material 316 and the sample material 316 thereby remains essentially bound to the membranes 306 unless and until the gel 102 is activated. This diffusion-isolation or releasable retention of sample material to the membranes 306 reduces the potential for cross-talk between the different samples applied to the different fingers 310 and loading areas 312 of the loader 308. Furthermore, contamination of the electrode buffer solution 408 is prevented using the present loader 308. After the sample material 316 is applied to the loading area 312 of the fingers 310, the membranes 306 bind the sample material to the loader 308 and thereby prevent the inadvertent elution of sample material into the electrode buffer solution 408 when the sample material 316 is placed in contact with the gel 102.
The present sample loader 308 of FIGURES 3a and 3b and used in the vertical EGS 400 of FIGURE 4 facilitates the efficient, accurate, inexpensive, and rapid insertion of sample material into a gel for gel electrophoresis. In contrast to the prior art sample loaders described above, little technical skill or dexterity is required to load samples into an EGS using the present sample loader. Samples can be quickly applied to the fingers 310 and more specifically the membranes 306 of the loader 308 before the loader 308 is placed in contact with the gel 102. Furthermore, because the loader 308 remains in contact with the gel 102 during the electrophoresis process, the structural integrity problems associated with the sample wells formed by the prior art sample loaders are eliminated. Moreover, undesirable sample material such as urea can be easily and quickly removed using the present sample loader. In contrast, as described above, the removal of undesirable sample material from the sample wells formed by the prior art sample loaders is a difficult and time-consuming process. Thus, the present sample loader 308 overcomes many of the drawbacks associated with the prior art sample loading devices and methods.
FIGURES 5a and 5b show the sample loader of FIGURES 3a and 3b intended for use in the horizontal EGS 200 described above with reference to FIGURES 2a and 2b. As shown in FIGURE 5a, the gel 204 is cast between two removable dams 202 before the insertion of sample material into the gel 204. After the gel 204 congeals, the dams 202 are removed from the device 200.
The device 200 is then filled with electrode buffer solution 408 to a level 1 16 which just exceeds an upper surface 220 of the gel 204. After the device 200 is filled with the electrode buffer solution 408 to the level 1 16, sample material 316 is applied to the loading areas 312 and the membranes 306 of the sample loader 308 as described above with reference to FIGURES 3a and 3b. The sample loader 308 is then positioned within the EGS 200 so that the loading areas 312 of the fingers 310 are positioned proximate a top edge 314 of the gel 204. Thus, the sample material 316 contacts the gel 204 at the upper edge 314 as shown in FIGURE 5b. As described above, the membranes 306 diffusion-isolate the sample material so that the sample material is reversibly bound to the membranes 306. Consequently, very little of the sample material diffuses into the gel 204 until the gel is activated by a release mechanism. An electric field is then applied to the gel 204 via the cathode wire 206 and anode wire 208 as described above with reference to FIGURE 2b. The biomolecular samples are then substantially released by the loader 308 and loaded into the gel 204.
FIGURE 6a shows details of a preferred embodiment of the sample loader of the present invention. As shown in FIGURE 6a, the sample loader 500 preferably comprises a substrate 502 and a plurality of fingers 504. A lower portion of the substrate 502 includes a membrane 506 which diffusion-isolates applied sample material by reversibly binding the sample material to the fingers 504 of the sample loader 500. The thickness of the membrane 506 may be varied to hold different sample amounts. Sample loading areas 512 can be further defined in the fingers 504 by a plurality of sample inhibiting agents 514 which are formed through the membrane 506. For example, the sample inhibiting agent 514 may comprise hydrophobic ink which extends through each membrane 506 to the substrate 502 across the proximal end of each finger 504, as shown. The hydrophobic ink 514 inhibits the migration or diffusion of sample material from one finger 504 to another. The position of the ink 514 on each finger may also be used to define and control the size of the sample loading area of the membranes 506.
Alternatively, the hydrophobic ink 514 can be positioned within the membrane 506 in any configuration which inhibits the inadvertent diffusion of sample material from one finger 504 to another. For example, as shown in FIGURE 6a, the hydrophobic ink 514' is vertically formed through the membrane 506 so that the ink 514' is equidistant between the fingers 504. As described above, the membrane 506 preferably comprises material which diffusion-isolates or reversibly binds the biomolecular sample material before activation of a release mechanism, such as the application of an electric field. The material preferably binds and substantially retains the sample material to the loading area 512 when it is immersed in a standard electrophoretic buffer solution. However, when an electric field is applied to the buffer solution, the membrane 506 preferably releases a substantial portion of the bound sample material into the gel for separation and identification. After applying an electric field to the gel, the sample transfer rate from the loading areas 512 to the gel is preferably substantially equivalent to the transfer rates between the sample wells and the gels in the prior art apparatuses. The resolution of the sample bands produced using the present loader 500 and the resolution of the sample bands produced using the prior art apparatuses are also preferably substantially equivalent. Any membrane material which meets these requirements can be used to implement the membrane of the present invention. However, a number of factors can affect the performance and therefore the selection of membrane material.
One factor which affects the selection of membrane material for use with the present sample loader is the type of samples which are to be applied to the membrane. The sample type can affect the membrane's ability to releasably bind and retain the sample. For example, DNA molecules appear to be more easily bound and retained by the membranes investigated than are RNA molecules. Similarly, using both native and denaturing conditions, proteins are less effectively bound and retained by the membranes than are DNA molecules. However, the RNA samples generally are released into the gel solution upon activation just as effectively as are the DNA samples. Also, the membrane's performance can vary under varying conditions of buffer solution pH, temperature, salt concentration, and strength. These varying conditions can affect the amount of electric charge required to fully release the samples from the membrane 506. Moreover, pre-wetting, pre-spotting. and drying time for pre-treated membranes, varying sample volume and the magnitude of the electric field applied to the buffer solution, can also affect membrane performance. The membrane 506 shown in FIGURE 6a preferably is used to load any type of biomolecular sample into an electrophoretic gel under typical laboratory conditions.
Taking the factors described above into consideration, the membrane preferably comprises either nitrocellulose or nylon. The nylons may either be electrically neutral, or positively or negatively charged. Among the samples preferably loaded by the present sample loader 500 are double-stranded DNA (dsDNA), single-stranded DNA (ssDNA), RNA, and proteins. The composition of the membrane 506 depends upon the samples to be loaded by the present sample loader. For example, when performing electrophoresis of dsDNA and RNA samples, the membrane 506 preferably comprises either neutral nylon or nitrocellulose. Examples of neutral nylons include Biotrans® available from ICN. located in Costa Mesa, CA., and Immobilon-S® available from Millipore, located in Bedford, MA. Examples of nitrocellulose materials include BA85 available from Schleicher & Schuell, located in Keene, NH, and Bioblot-NC® available from Costar, located in Cambridge, MA.
Alternatively, nitrocellulose membranes are preferred when performing electrophore¬ sis of ssDNA and sequencing reactions. When proteins are to be loaded into a gel of an EGS, the membrane 506 preferably comprises Teflon® or polyvinylidene fluoride (PVDF) nylon.
Although some specific sample and membrane materials have been described, they should not be taken as limiting the scope of the present invention. The present invention contemplates the use of any membrane which adequately releasably binds and retains sample material before activation of a release mechanism, yet which efficiently releases a substantial portion of the sample material into the gel after the system is activated by a release mechanism.
Referring again to FIGURE 6a, the present sample loader 500 preferably includes a substrate 502 which structurally supports the membrane 506. The substrate 502 preferably comprises a non-conductive, relatively inert, non-porous, neutrally charged, inexpensive material. The substrate preferably comprises either celluloid or plastic. The substrate 502 may be manufactured using a number of techniques. For example, the substrate 502 may first be cut to a desired width. The fingers 504 may then be formed in one side of the substrate 502 by cutting, scoring or punching away areas 520 between the fingers 504. Preferably, the fingers 504 are formed sufficiently long to prevent capillary action or wicking of buffer solution from contaminating the samples applied to the membrane loading areas. Similarly, the fingers 504 are preferably sufficiently long to prevent wicking of a sample from a first loading area 512 to a second loading area 512 on another finger 504.
Preferably, the present sample loader 500 is manufactured by placing the substrate 502 (which is typically formed into strips) into a membrane slurry material. The membrane slurry is placed in contact with the substrate 502 until it solidifies upon the surface of the substrate. The fingers 504 are formed in the substrate by punching or cutting away areas between the fingers. Sample loading areas 512 are defined in the fingers 504 by scoring substantially horizontal lines across approximate midpoints of the fingers 504. During the scoring process, the solidified membrane material is cut away from the substrate 502. The substrate 502 is left in tact. In one preferred embodiment, the scored membrane is filled with hydrophobic ink 514 as shown in FIGURE 6a and described above. Other alternative embodiments use photoetching or photomasking techniques to define the sample loading areas 512.
The membrane 506 may be formed on the finger side of the substrate 502 by any convenient method, such as screening liquid membrane material to the substrate 502 or dipping the substrate 502 into a liquid membrane pool for a time which is sufficient to allow the membrane material to adhere to the substrate 502. Alternatively, the membrane may be formed by cutting membrane bulk material into strips of equal widths and affixing the strips on the substrate 502 as shown in FIGURE 6a. That is, the strips of membrane can be used to define the fingers 504 of the sample loader 500. In one preferred embodiment, the membrane comprises sheets of plastic-backed nitrocellulose material available from Schleicher & Schuell. As described above with reference to FIGURE 3a, one alternative embodiment of the sample loader 500 shown in FIGURE 6a eliminates the necessity for the substrate 502. If the membrane 506 comprises material which is sufficiently rigid, and if the membrane 506 is sufficiently thick, the entire substrate 502 can be replaced with membrane material (i.e., the membrane 506 is used as the substrate). The fingers 504, sample loading areas 512, and sample inhibiting agents 514 (if necessary) are formed into the membrane as described above with reference to the preferred embodiment. Also, in another alternative embodiment shown in side view in FIGURE 6b, the substrate 502 is substantially thicker than the substrate of the preferred embodiment and the membrane 506. In this alternative embodiment, the relatively thin membrane 506 and fingers 504 are attached as "legs" to the bottom 503 of the substrate 502.
FIGURE 6c shows a front plan view of yet another alternative embodiment of the present invention. The embodiment of FIGURE 6c is similar to that shown in FIGURE 6a with the exception that the fingers 504 have been replaced by "virtual fingers" which are formed into the substrate 502'. The sample loader 500' shown in FIGURE 6c is preferably manufactured by screening membrane material 506' onto a sample loading portion of the substrate 502' and thereby creating sample loading areas 512' (or "virtual fingers") onto the substrate 502'. As described above with reference to FIGURE 6a. the sample loading areas 512' diffusion-isolate sample material which is applied thereto until the membrane 506' is activated by a release mechanism. The notches 520 of FIGURE 6a are replaced by the virtual notches 520' which are merely areas of diffusion-isolation between the sample loading areas 512'. The embodiment shown in FIGURE 6c is useful in EGS applications which do not require sample loading fingers which extend downwardly toward the EGS gel.
The alternative embodiment shown in FIGURE 6c can alternatively be manufactured by first applying or affixing membrane material to the sample loading portion of the substrate 502'. and then scoring the membrane 506' to create the virtual notches 520' (i.e., areas where membrane material is removed from the substrate 502') as shown in FIGURE 6c. Alternatively, the sample loading areas 512' can be diffusion-isolated from each other using a chemical isolation means such as the hydrophobic ink described above with reference to FIGURE 6a. If hydrophobic ink is used, the loading areas 512' can be formed by first deeply scoring into the membrane 502' and thereafter filling the scored portions of the substrate with the ink.
Other alternative embodiments of the present sample loader are shown in FIGURES 7 and 8. FIGURE 7 shows an end-loaded sample loader 600. Similar to the sample loader of FIGURE 6a. the end-loaded sample loader 600 preferably includes a substrate 502, a plurality of teeth or sample loading fingers 504, each having a proximal end 602 and a distal end 604, wherein the fingers extend downwardly away from the proximal end 602, a sample loading area 512 at the distal end 604 of the fingers 504, and a membrane 606. The membrane 606 is affixed to the distal end 604 of the fingers 504 so that only a very small percentage of the total finger length is covered by the membrane 606. In contrast, as described above, the membrane 506 of the sample loader 500 of FIGURES 6a and 6b covers a substantial length of the fingers. Using the end-loaded sample loader 600 of FIGURE 7. sample material is applied to the sample loading areas 512 by simply dipping or otherwise adhering the sample material to the membranes 606. For conventional EGS, the membrane 606 should be sufficient to hold a sample in solution where the drop volume is at least approximately 0.3 μL.
If the fingers 504 are sufficiently long, the loader does not require use of a sample inhibiting agent such as the hydrophobic ink described above with reference to the preferred embodiment shown in FIGURE 6. Because a sample is applied only to the distal end 604 of a finger 504, and not along the entire length of the finger, the sample is less likely to diffuse from one finger to either the buffer solution or another finger.
Therefore, the longer the fingers 504, the less potential for sample or buffer contamination and cross-talk. However, an alternative end-loaded sample loader might include such a sample inhibiting agent similar to that described above with reference to FIGURE 6. As described above, if included, the sample inhibiting agent preferably comprises hydrophobic ink which inhibits the migration or diffusion of sample material from one finger 604 to another. The ink is preferably positioned across the width of each finger 504 at the proximal ends 602 of the fingers 504. As described above with reference to the preferred embodiment, the membrane 606 can alternatively serve as its own substrate.
FIGURE 8 shows another alternative embodiment of the end-loaded sample loader of FIGURE 7. Similar to the loader of FIGURE 7, the sample loader shown in FIGURE 8 preferably includes a substrate 502, and a plurality of sample loading fingers 504, each having a proximal end 702 and a distal end 704, wherein the fingers 504 extend downwardly away from the proximal end 702. The fingers 504 include a three- dimensional sample loading area 712 which surrounds the distal end 704 of the fingers 504. The sample loading areas 712 are preferably formed by dipping the fingers 504 into a pool of membrane material, removing the loader 700 from the pool of membrane material, and allowing the membranes to solidify into the colloidons shown in FIGURE 8. Because the loading areas 712 are much more three-dimensional than the rectangularly-shaped loading areas 512 of the sample loader shown in FIGURE 7 (the loading areas 512 are substantially two-dimensional), the loading areas 712 accommodate a greater volume of sample material than do the loading areas 512.
Before insertion of the sample loader fingers 504 into a gel of an EGS, samples are typically applied to the membranes covering the sample loading areas 712 and allowed to dry. Similar to the sample loader of FIGURE 7. if the fingers 504 are sufficiently long, a sample inhibiting agent need not be used. Because samples are applied only to the sample loading areas 712, the samples are less likely to diffuse from one finger to another and thereby cause cross-contamination of samples. However, as with the loader of FIGURE 7. an alternative end-loaded sample loader might include sample inhibiting agents similar to those described above with reference to FIGURES 6a and 6b.
All of the embodiments of the present invention of an apparatus and method of loading samples into a gel of an EGS may also be used with the prior art systems which first form sample wells in the gels and then load the wells with the samples to be tested. The present invention may be used to load sample material into the sample wells after the gel polymerizes. Alternatively, the present invention may be used to load samples into sample wells previously formed by a prior art well-forming device.
Thus, in essence, the present invention is a sample loader for an EGS having well- defined diffusion-isolated sample loading areas. The sample loading areas preferably include a membrane which releasably retains applied sample material until and unless the membrane is activated by a release mechanism. When immersed in a buffer solution and/or gel of an EGS, the sample material sufficiently adheres to the membrane so that the sample material does not diffuse substantially into the gel before activation of a release mechanism. However, when activated by a release mechanism, the membrane releases a substantial portion of the sample material into the gel and allows the sample material to undergo an electrophoretic process. A number of different means may be used to diffusion-isolate the loading areas. For example, the loading areas may be chemically-isolated using a hydrophobic ink. Alternatively, the substrate of the loader may be scored thereby forming "virtual fingers" in the substrate. Hydrophobic ink may alternatively be used to fill in the scored areas and thus further diffusion-isolate the virtual fingers.
A number of embodiments of the present invention have been described. Neverthe¬ less, it will be understood that various modifications may be made without departing from the spirit and scope of the invention. For example, as described above, all of the embodiments of the present invention may use membrane material as the substrate of the loaders. Further, the shape of the various loaders described above and shown in the figures is exemplary only, and is not intended to restrict the scope of the invention. For example, although the fingers 504 (FIGURES 6-8) are rectangular in the embodiments shown and described, they could also be substantially pyramidical, spherical, cylindrical, parallelogram-like or triangular. Similarly, the fingers 504 can be longer or shorter depending upon the application. The shape of the substrate can also be alternatively modified. For example, the side of the sample holder which is grasped by a technician may be circularly-shaped, or may include a handle for easy handling. The width of the fingers and membranes can also be varied depending upon the amount of sample material to be loaded. Also, the loader can be manufactured by arranging parallel sheets of substrate under a single membrane sheet, and adhering the membrane to both sides of the substrates. Each parallel sheet thereby forms a finger of the sample loader. Furthermore, although the method of using the present sample loader discloses placing the sample loading areas into contact with the electrophoretic gel material, the present sample loader can also be used by inserting the sample loading areas and fingers into the gel.
Accordingly, it is to be understood that the invention is not to be limited by the specific illustrated embodiment, but only by the scope of the appended claims.

Claims

1. A sample applicator, for use in an electrophoretic gel system, comprising:
(a) at least one sample loading area configured to be placed in contact with a gel in an electrophoretic gel system, the sample loading area comprising a membrane capable of releasably retaining an applied sample;
(b) wherein a useful portion of the sample is actively released from the membrane when the membrane is placed in contact with the gel in an electrophoretic gel system in the presence of a release mechanism.
2. The applicator of claim 1, wherein the applied sample is releasably retained by the membrane while the membrane is immersed in an electrophoretic gel system buffer solution.
3. The applicator of claim 1 , wherein the release mechanism does not substan¬ tially affect the electrophoretic action of the electrophoretic gel system.
4. The applicator of claim 1 , wherein the applied sample is releasably retained by the membrane while the membrane is inserted into the gel until activation by the release mechanism.
5. The applicator of claim 1. further comprising a sample inhibiting agent formed through the membrane, wherein the sample inhibiting agent prevents the diffusion of samples away from the sample loading area.
6. The applicator of claim 1. wherein the sample inhibiting agent comprises hydrophobic ink.
7. An apparatus for loading samples into a gel immersed in an electrode buffer solution for use in an electrophoretic gel system, comprising:
(a) a substrate having at least one sample loading area; and
(b) a membrane adhered to the sample loading area, wherein the mem- brane is capable of reversibly binding an applied sample, and wherein a substantial portion of the sample is released from the membrane when the membrane is placed in contact with the gel and the gel is activated by a release action.
8. The apparatus of claim 7, wherein substantially all of the applied sample is reversibly bound by the membrane while the membrane is immersed in an electrode buffer solution.
9. The apparatus of claim 7, wherein substantially all of the applied sample is reversibly bound by the membrane while the membrane is inserted into the gel until activation by the release action.
10. The apparatus of claim 7. wherein the release action does not substantially affect the performance of the electrophoretic gel system.
1 1. The apparatus of claim 7. wherein the substrate is non-conducting, substan¬ tially inert, non-porous, and neutrally charged.
12. The apparatus of claim 7, wherein the substrate comprises a material selected from the group consisting of celluloid and plastic.
13. The apparatus of claim 7. wherein the membrane comprises a material selected from the group consisting of nitrocellulose and nylon.
14. The apparatus of claim 7. wherein the membrane comprises a material selected from the group of electrically neutral nylon, positively charged nylon and negatively charged nylon.
15. The apparatus of claim 7. wherein the membrane reversibly binds the applied sample via absorption of the sample to the membrane.
16. The apparatus of claim 7. wherein the membrane reversibly binds the applied sample by restricting the capillary action of the sample.
17. The apparatus of claim 7, wherein the membrane reversibly binds the applied sample via an ionic affinity between molecules of the membrane and the applied sample.
18. The apparatus of claim 7, wherein the membrane reversibly binds the applied sample via biomolecular affinity between the membrane and the applied sample.
19. The apparatus of claim 7, wherein the release action comprises applying an electric field to the electrode buffer solution.
20. The apparatus of claim 7, wherein the release action comprises varying the temperature of the buffer solution.
21. The apparatus of claim 7, wherein the release action comprises varying the pH balance of the electrode buffer solution.
22. The apparatus of claim 7, wherein the release action comprises varying the magnitude of an electric charge applied to the buffer solution.
23. The apparatus of claim 7. wherein the release action comprises applying an electromagnetic field to the buffer solution.
24. The apparatus of claim 7, wherein the release action comprises varying the strength of the buffer solution.
25. The apparatus of claim 7, wherein the release action comprises varying a salt concentration of the buffer solution.
26. The apparatus of claim 7, wherein the release action comprises irradiating the buffer solution.
27. The apparatus of claim 7, wherein the release action comprises exposing the buffer solution to particle bombardment.
28. The apparatus of claim 7, wherein the release action comprises applying sonic waves to the buffer solution.
29. The apparatus of claim 7, further comprising a sample inhibiting agent formed through the membrane, wherein the sample inhibiting agent prevents the diffusion of samples away from the sample loading area.
30. A method of loading samples into a gel of an electrophoretic gel system, comprising the steps of:
(a) applying a sample to a respective membrane of a sample loader, wherein each membrane releasably retains each sample until activation of a release mechanism;
(b) activating the release mechanism; and
(c) releasing an effective portion of each sample into the gel for gel electrophoresis.
31. The sample loading method of claim 30, wherein the sample loader includes a substrate and a plurality of sample loading fingers, and wherein the membrane is affixed to the substrate to substantially cover the fingers.
32. The sample loading method of claim 30, wherein the membrane comprises a material selected from the group consisting of nitrocellulose and nylon.
33. The sample loading method of claim 30, wherein the substrate comprises a material selected from the group consisting of celluloid and plastic.
34. The sample loading method of claim 30, wherein the membrane releasably retains each sample to the loader by absorption of each sample to the membrane.
35. The sample loading method of claim 30, wherein the membrane reversibly binds each applied sample by restricting the capillary action of each sample.
36. The sample loading method of claim 30. wherein the membrane reversibly binds each applied sample via an ionic affinity between molecules of the membrane and each applied sample.
37. The sample loading method of claim 30, wherein the membrane reversibly binds each applied sample via biomolecular affinity between the membrane and each applied sample.
38. The sample loading method of claim 30, wherein the release mechanism comprises applying an electric field to the electrode buffer solution.
PCT/US1996/002982 1995-03-03 1996-03-01 Membrane loader for gel electrophoresis WO1996027787A1 (en)

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AU54189/96A AU5418996A (en) 1995-03-03 1996-03-01 Membrane loader for gel electrophoresis
EP96911246A EP0871870A1 (en) 1995-03-03 1996-03-01 Membrane loader for gel electrophoresis

Applications Claiming Priority (2)

Application Number Priority Date Filing Date Title
US39789895A 1995-03-03 1995-03-03
US08/397,898 1995-03-03

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Cited By (9)

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WO1998030911A2 (en) * 1997-01-10 1998-07-16 Europäisches Laboratorium für Molekularbiologie (EMBL) Sample transfer
WO1999012025A1 (en) * 1997-09-01 1999-03-11 Medical Research Council Gel loading
US5939022A (en) * 1997-12-09 1999-08-17 Pharmacia Biotech, Inc. Article for transporting biological samples during analysis
EP0971229A1 (en) * 1998-07-10 2000-01-12 LION Bioscience AG Method for introducing a sample, introducing means and electrophoretic apparatus
EP0976758A1 (en) * 1998-07-10 2000-02-02 LION Bioscience AG Use of porous membranes, either neutrally or negatively charged, as a loading material for gel electrophoresis
US6406602B1 (en) 1998-12-23 2002-06-18 Genome Therapeutics Corporation Sample loading device for gel electrophoresis
US6544395B1 (en) * 1996-05-06 2003-04-08 Helena Laboratories Corporation System for the application of samples on a substrate
WO2005062032A1 (en) * 2003-12-23 2005-07-07 Ge Healthcare Bio-Sciences Ab Novel use of positively charged support
ES2326504A1 (en) * 2006-08-11 2009-10-13 Universidad Del Pais Vasco- Euskal Herriko Unibersitatea (80%) Method for loading samples for submerged agarose gel electrophoresis

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US4334879A (en) * 1979-05-04 1982-06-15 Olympus Optical Co., Ltd. Sample applicator
US5405516A (en) * 1991-01-04 1995-04-11 Sebia Apparatus for the application of biological samples to an electrophoretic slab support

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US4334879A (en) * 1979-05-04 1982-06-15 Olympus Optical Co., Ltd. Sample applicator
US5405516A (en) * 1991-01-04 1995-04-11 Sebia Apparatus for the application of biological samples to an electrophoretic slab support

Cited By (13)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US6544395B1 (en) * 1996-05-06 2003-04-08 Helena Laboratories Corporation System for the application of samples on a substrate
US6428668B1 (en) 1997-01-10 2002-08-06 Europaisches Laboratorium Fur Molekularbiologie (Embl) Sampler transfer
WO1998030911A3 (en) * 1997-01-10 1998-11-12 Europ Lab Molekularbiolog Sample transfer
WO1998030911A2 (en) * 1997-01-10 1998-07-16 Europäisches Laboratorium für Molekularbiologie (EMBL) Sample transfer
WO1999012025A1 (en) * 1997-09-01 1999-03-11 Medical Research Council Gel loading
US5939022A (en) * 1997-12-09 1999-08-17 Pharmacia Biotech, Inc. Article for transporting biological samples during analysis
DE19830989C1 (en) * 1998-07-10 2000-04-13 Lion Bioscience Ag Use of porous membrane materials as loading materials in gel electrophoresis
EP0976758A1 (en) * 1998-07-10 2000-02-02 LION Bioscience AG Use of porous membranes, either neutrally or negatively charged, as a loading material for gel electrophoresis
EP0971229A1 (en) * 1998-07-10 2000-01-12 LION Bioscience AG Method for introducing a sample, introducing means and electrophoretic apparatus
US6406602B1 (en) 1998-12-23 2002-06-18 Genome Therapeutics Corporation Sample loading device for gel electrophoresis
WO2005062032A1 (en) * 2003-12-23 2005-07-07 Ge Healthcare Bio-Sciences Ab Novel use of positively charged support
AU2004304217B2 (en) * 2003-12-23 2010-04-22 Ge Healthcare Bio-Sciences Ab Novel use of positively charged support
ES2326504A1 (en) * 2006-08-11 2009-10-13 Universidad Del Pais Vasco- Euskal Herriko Unibersitatea (80%) Method for loading samples for submerged agarose gel electrophoresis

Also Published As

Publication number Publication date
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