Classifications

• • G—PHYSICS
  • G01—MEASURING; TESTING
  • G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
  • G01N27/00—Investigating or analysing materials by the use of electric, electrochemical, or magnetic means
  • G01N27/26—Investigating or analysing materials by the use of electric, electrochemical, or magnetic means by investigating electrochemical variables; by using electrolysis or electrophoresis
  • G01N27/416—Systems
  • G01N27/447—Systems using electrophoresis
  • G01N27/44756—Apparatus specially adapted therefor
• • G—PHYSICS
  • G01—MEASURING; TESTING
  • G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
  • G01N27/00—Investigating or analysing materials by the use of electric, electrochemical, or magnetic means
  • G01N27/26—Investigating or analysing materials by the use of electric, electrochemical, or magnetic means by investigating electrochemical variables; by using electrolysis or electrophoresis
  • G01N27/416—Systems
  • G01N27/447—Systems using electrophoresis
  • G01N27/44704—Details; Accessories
  • G01N27/44717—Arrangements for investigating the separated zones, e.g. localising zones

Definitions

• the present invention relates to an electrophoretic separation apparatus for separating and separating substances such as proteins mixed in an electrophoresis solution by electrophoresis.
• substances such as proteins are fractionated by electrophoresis according to charge and molecular weight, and fractionated components are each fractionated by means of a preparative capillary electrophoresis apparatus, a preparative liquid electrophoresis apparatus, or the like.
• a point electrophoresis apparatus a method of extracting a target substance from the gel after electrically separating in a gel, and the like.
• these devices and methods had the following problems.
• the preparative type capillary electrophoresis apparatus has electrodes arranged at both ends of a linear capillary with a diameter of 1 mm or less, and has very high separation ability (fractionation ability).
• separation ability fractionation ability
• the separation of substances separated by isoelectric focusing is performed at the end of the capillary, it is necessary to extrude the separated substances from the capillary. This extrusion operation has the disadvantage of disturbing the separation pattern, so that high-precision fractionation cannot be performed.
• the diameter of the capillary is as small as 1 mm or less, the amount of the sample that can be subjected to electrophoresis is small, and therefore, a large amount is required for one operation such as structural analysis of amino acid sequences. There was a drawback that it was not suitable for an electrophoresis step that required a sample.
• the preparative liquid isoelectric focusing apparatus is designed to perform isoelectric focusing in a cylinder whose interior is divided into 20 fractions by a membrane. This Since the electrophoresis is performed in the electrophoresis tube partitioned by the membrane as described above, even after the energization is stopped, the diffusion of the substance after the separation is suppressed, and there is no disadvantage of the preparative-type capillary electrophoresis apparatus described above. However, since the number of fractions was only 20, there was a disadvantage that the resolution was slightly inferior and high-precision fractionation could not be performed. In addition, there was a problem that adsorption of proteins to the membrane and clogging of the membrane due to isoelectric precipitation adversely affect the separation ability.
• the method of extracting the target substance from the gel is as follows: the gel prepared with polyacrylamide, etc. is used as an electrophoresis solution, electrophoresis is performed, and the target substance is identified by staining the sample after electrophoresis.
• This is a method of extracting and extracting a gel containing the target substance. Depending on the size of the gel, a large amount of several mg of sample can be added and the resolving power is relatively high.However, since an operation to extract the target substance separated by electrophoresis from the gel is required, the extraction efficiency is low. However, there were problems such as lowering of the water content and mixing of contaminants from the gel.
• An object of the present invention is to provide an electrophoresis apparatus which has high resolution and enables high-precision separation with a simple operation. .
• the present invention provides an electrophoretic separation apparatus, wherein a plurality of independent cells are provided on a contact surface of two members joined to be relatively movable with each other, and the two members are moved by relative movement. A position in which a large number of cells are independently maintained and a position in which the large number of cells are connected to one electrophoresis passage are alternately switchable.
• electrodes are arranged at both ends It is assumed that.
• the two members can be switched alternately between a position where many cells are connected to each other to form a single electrophoresis passage and a position where they remain independent.
• the electrophoresis is performed at a position where an electrophoresis passage connected to one is formed, and the electrophoresis passage is filled with an electrophoresis solution (carrier ampholyte) containing a substance to be fractionated, the electrophoresis is performed as described above.
• the substance can be fractionated at the position of each isoelectric point.
• these two members are switched to a position where each cell becomes an independent state, the substance separated at each isoelectric point by the switching operation is obtained. Since each cell is independently confined in each cell, high-precision fractionation can be performed for each cell.
• the substance fractionated at each isoelectric point can be collected and can be performed regardless of the diameter of the electrophoresis passage.
• the sample can be processed.
• the substance applicable to the electrophoretic separation device of the present invention is not particularly limited as long as it is an electrophoretic substance. That is, the substance is, of course, a substance having a charge, such as a protein, but even if it is an uncharged organic compound, a substance having a charge, such as a surfactant, is put into an electrolytic solution to form a whole.
• the present invention can be applied to a state having electric charge.
• As the protein a polypeptide of a dipeptide or higher can be applied.
• the separation accuracy can be further improved. This makes it possible to separate cells and separate DNA (deoxyribonucleic acid), which can also be used for sperm selection when separating men and women.
• FIG. 1 is a plan view showing an example of the electrophoretic separation device of the present invention.
• FIG. 2A is a cross-sectional view showing a state in which a large number of cells in the electrophoretic separation device of FIG.
• FIG. 2B is a cross-sectional view taken along the line Hb-Hb in FIG. 2A.
• FIG. 3A is a cross-sectional view showing a state where the zigzag electrophoresis passage of FIG. 2A is separated into a plurality of independent cells.
• FIG. 3B is a cross-sectional view taken along arrow IE b—El b in FIG. 3A.
• FIG. 4A is a cross-sectional view showing an embodiment in which the cells in the electrophoretic separation device of FIG. 1 are enlarged in the depth direction as shown in FIG. 4B.
• FIG. 4B is a sectional view taken along the line Wb-IVb in FIG. 4A.
• FIG. 5A is a cross-sectional view of an embodiment in which the pitch of cells forming a zigzag electrophoresis passage is reduced.
• FIG. 5B is a cross-sectional view taken along the line Vb-Vb in FIG. 5A.
• FIG. 6 is a vertical cross-sectional view showing a state in which the slider in the state of FIGS. 5A and 5B is moved up and down to separate the zigzag-shaped electrophoresis passage into a plurality of independent cells.
• FIG. 7 is a plan view partially showing a main part of an electrophoretic separation apparatus according to another embodiment of the present invention.
• FIG. 8 is a plan view showing, in partial cross section, a state in which one electrophoresis passage in the electrophoresis separation apparatus of FIG. 7 is changed to a plurality of independent cells.
• FIG. 9A is a front view showing a main part of an electrophoretic separation device according to still another embodiment of the present invention.
• FIG. 9B is a plan view of FIG. 9A.
• the electrophoresis separation apparatus of the present invention shown in FIG. It is mounted in the support frame 3 in a state of being in close contact with each other.
• the step 1 and the slider 2 are preferably made of a colorless and transparent material such as acrylic resin or quartz glass that allows the inside to be seen from the outside.
• the slider 2 While the stay 1 is fixed in the support frame 3 so as not to move, the slider 2 is obtained by removing the spacer 4 with the spacer 4 interposed at one end in the longitudinal direction. It slides in the longitudinal direction. The slider 2 is pressed by the panel 5 held by the screw 7 screwed to the support frame 3 so as to be in close contact with the stay 1 side, and is further screwed to the support frame 3 in the longitudinal direction. The panel 6 held by the screw 8 is pressed toward the spacer 4 side.
• a number of cells 10 bent in an inverted V shape are formed at a constant pitch in the longitudinal direction.
• a large number of cells 11 bent in a V-shape are formed at the same pitch in the longitudinal direction.
• These cells 10 and 11 may have any size, for example, a V-shape It is recommended that the total length be 10 mm, the cross-sectional diameter be 1.5 mm, and the angle between the V-shaped vertices be about 60 °.
• storage rooms 12 and 13 are provided at both ends in the longitudinal direction so as to open to the upper surface side of the stay 1, and the storage rooms 12 and 13 of the brackets are respectively arranged on the outermost side.
• the cells are connected to the cells 10 and 10 located at both ends. Electrodes 14 (cathode) and electrode 15 (negative electrode) are attached to the storage chambers 12 and 13, respectively. Connected via switch 19.
• the cell 10 on the station 1 side and the cell 11 on the slider 2 side are connected as shown in FIGS. 2A and 2B.
• One zigzag electric swimming path P is connected alternately with each other.
• the spacer 4 is removed and the slider 2 is slid in the longitudinal direction, the cells 10 and 11 are separated from each other as shown in FIGS. 3A and 3B, and each is switched to an independent state. It is like that.
• Separation holes 16 and 17 are connected to the cells 10 and 11, respectively, and are provided so as to open to the upper surfaces of the stage 1 and the slider 2. Plugs 16a and 17a are detachably attached to the sorting holes 16 and 17, respectively, as necessary. Therefore, the material fractionated by the electrophoresis can be easily separated by using a pipe or the like for each cell via the separation holes 16 and 17.
• the electrophoretic fractionation apparatus of the present invention when fractionation and fractionation of proteins is performed by the above-described electrophoretic fractionation apparatus of the present invention, first, as shown in FIGS. A number of cells 11 on the side are connected to each other to form one zigzag electrophoresis passage P. Next, the electrophoresis passage P is filled with an electrophoresis solution (carrier ampholyte) containing one or more types of proteins, and the storage chamber 12 is further filled with an alkaline solution. Fill 13 with acidic solution.
• electrophoresis solution carrier ampholyte
• the electrophoresis operation multiple cells are connected to one electrophoresis passage P.
• the two members are moved relative to each other to make the above-mentioned cells independent, so that high-precision sorting can be performed without disturbing the pattern separated by electrophoresis.
• the material separated by electrophoresis can be accurately separated by a simple operation of simply moving the two members relative to each other. Irrespective of temperature, it is possible to process a large number of samples at once.
• FIGS. 4A and 4B show an embodiment in which the capacity of each cell can be increased without changing the number of sections of the cells 10 and 11.
• the cross-sectional area of each cell is increased by increasing the depth without changing the pitch between cells.
• the amount of sample that can be processed at one time can be increased.
• FIGS. 5A and 5B show an embodiment in which the division pitch p of the cells 10 and 11 is further reduced to increase the number of cell sections and improve the resolution.
• the cells 10 and 11 are mutually independent by setting the slide direction of the slider 2 to a direction intersecting the vertical direction, that is, a direction intersecting the longitudinal direction as shown in FIG. It is made to be in a state.
• the members constituting the stay 21 and the slider 22 each have a large number of laminated plates 21a and 22a, and the laminated plates 21a and 22a have cells 30 and 31 formed of through holes. Is provided. These cells 30 and 31 are provided with sorting holes 16 and 17, respectively.
• the stay 21 and the slider 22 are combined so that the laminated plates 21a and 22a are alternately stacked.
• the cell 30 of the stay 21 and the cell 31 of the slider 22 are arranged as shown in FIG. Are connected to each other to form one linear electrophoresis passage P, and by moving the slider 22 in the direction of the arrow as shown in FIG. 8, the cell 30 of the station 21 and the slider 22 are moved.
• cell 31 can be switched to a position where they are independent of each other. Therefore, according to the electrophoretic fractionating apparatus of this embodiment, the same electrophoretic fractionation and fractionation as in the above-described embodiment can be performed.
• 9A and 9B illustrate yet another embodiment of the present invention.
• the members constituting the stay 41 and the slider 42 are formed of a cylindrical body and a rod-like body fitted therein.
• the cylindrical stay 41 is provided with a plurality of grooves 50 at a constant pitch in the longitudinal direction on the inner circumferential surface in contact with the rod-shaped slider 42.
• a plurality of grooves-shaped cells 51 are provided at the same pitch in the longitudinal direction so as to be offset from the above-mentioned cell 50 on the outer surface of the cylinder in contact with 4c.
• Separating mosquitoes L 16 and 17 are provided to communicate with
• the step 41 and the slider 42 move the slider 42 in the circumferential direction from the position where the cell 50 and the cell 51 are independent from each other as shown in FIGS. 9A and 9B.
• the electrophoretic fractionation apparatus of this embodiment can also perform the same electrophoretic fractionation and fractionation as in the above embodiment.
• the electrophoretic separation apparatus of the present invention two members having a large number of independent cells formed on contact surfaces that are in contact with each other are moved relative to one electrophoresis passage. Because it is possible to alternately switch between the position where it is connected to the cell and the position where it becomes independent, a large number of cells are formed in one electrophoresis passage and electrophoresis is performed, and then the cells are simply switched to the independent state. Materials separated by electrophoresis can be collected with high accuracy. Also, it is possible to process a large number of samples at once.
• the electrophoretic separation apparatus of the present invention can perform separation with higher separation accuracy by combining a substance separated and separated by this apparatus with a separation operation by chromatography. become.
• An electrophoretic separation apparatus having the configuration shown in Fig. 1 was manufactured, in which the total number of cells provided in the station and the cells provided in the slider was 61, and this electrophoretic separation apparatus was used. Electrophoretic fractionation of a standard protein between commercially available albumin and myoglobin was performed under the following conditions.
• albumin and myoglobin were separated into about three fractions each, and high-precision fractionation was possible.
• Electrophoresis solution 0.01% as a colorant in 4% amorphous
• Electrode bath liquid anode 0.1 mol H P ⁇ 4
• electrophoretic fractionation was performed under the following conditions using unpurified commercially available myoglobin as a sample to separate proteins with similar isoelectric points. went.
• Electrophoresis solution A solution in which 1% hydroxypropylmethylcellulose (HPMC) has been added to 4% unforeline to give a sharpness
• Electrode bath liquid anode 0.1 mol H 3 P ⁇ 4
• Electrophoretic fractionation was performed under the following condition I, and the sample was divided into 61 sections.
• each of the samples divided into 61 sections was placed on an autosampler, and further separated by liquid chromatography under the following condition H.
• the electrophoretic separation device of the present invention can be used for electrophoretic separation of a charged substance such as a protein.
• a charged substance such as a protein.
• it can be applied if a charged substance such as a surfactant is put in an electrolytic solution so as to have a charged state as a whole. is there.
• the present invention can also be used for cell sorting and DNA (deoxyribonucleic acid) separation.

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• Health & Medical Sciences (AREA)
• Life Sciences & Earth Sciences (AREA)
• Molecular Biology (AREA)
• Chemical & Material Sciences (AREA)
• Biochemistry (AREA)
• Electrochemistry (AREA)
• Physics & Mathematics (AREA)
• Analytical Chemistry (AREA)
• Chemical Kinetics & Catalysis (AREA)
• General Health & Medical Sciences (AREA)
• General Physics & Mathematics (AREA)
• Immunology (AREA)
• Pathology (AREA)
• Peptides Or Proteins (AREA)
• Electrostatic Separation (AREA)
• Apparatus Associated With Microorganisms And Enzymes (AREA)

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Cited By (12)

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• 1994
  • 1994-11-29 WO PCT/JP1994/001999 patent/WO1995014923A1/ja not_active Application Discontinuation
  • 1994-11-29 EP EP95901605A patent/EP0682248A1/en not_active Withdrawn
  • 1994-11-29 JP JP51496295A patent/JP3190347B2/ja not_active Expired - Fee Related
  • 1994-11-29 US US08/495,674 patent/US5609743A/en not_active Expired - Fee Related

Patent Citations (3)

Non-Patent Citations (1)

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