JP3781687B2 - Genetic diagnostic apparatus and genetic diagnostic method - Google Patents

Description

【図面の簡単な説明】
【図１】本発明の実施の形態１における遺伝子診断装置の外観図
【図２】本発明の実施の形態１における遺伝子診断装置の上蓋開放外観図
【図３】本発明の実施の形態１における遺伝子診断装置の装置構成図
【図４】本発明の実施の形態１における遺伝子診断装置の制御回路要部図
【図５】本発明の実施の形態１における遺伝子診断装置の密閉流路内の分離用ＤＮＡコンジュゲートと遅延用ＤＮＡコンジュゲートとＤＮＡ試料との導入状態図
【図６】（ａ）本発明の実施の形態１における遺伝子診断装置の密閉流路内の分離用ＤＮＡコンジュゲートとＤＮＡ試料との関係概念図
（ｂ）本発明の実施の形態１における遺伝子診断装置の密閉流路内の遅延用ＤＮＡコンジュゲートとＤＮＡ試料との関係概念図
【図７】経過時間と吸光度の関係図
【図８】本発明の実施の形態２における遺伝子診断装置の装置構成図
【符号の説明】
１ 電源スイッチ
２ 操作ボタン
３ 表示パネル
４ 上蓋
５ 筐体
６ 電気泳動部
７ 支持台
８ 制御演算部
９ 電源ボックス
９ａ 電源部
１０ 高温部
１１ 断熱部
１２ 分離部
１３ 第１温調器
１４ 第２温調器
１５ 検出部
１５ａ Ｄ₂ランプ
１５ｂ フォトダイオード
１５ｃ プリアンプ
１５ｄ Ａ／Ｄコンバータ
１６，１７ 電極
１８ 緩衝液
１８ａ，１８ｂ 容器
１８ｄ リニアポリマーゲル
１９ キャピラリー管
２０ 吸引ポンプ
２１ 分離用ＤＮＡコンジュゲート
２２ 遅延用ＤＮＡコンジュゲート
２３ ＤＮＡ試料[0001]
BACKGROUND OF THE INVENTION
The present invention relates to a genetic diagnostic apparatus and a genetic diagnostic method that can easily and accurately detect the presence or absence of a genetic abnormality.
[0002]
[Prior art]
All diseases involve genetic factors and environmental factors with various probabilities, but diseases such as congenital metabolic disorders, cancer, diabetes, hypertension, Alzheimer, autoimmune diseases, atopy, obesity, and alcoholism Hereditary factors account for a very large proportion. On the other hand, diseases that have a large contribution of environmental factors include diseases caused by infections and aftereffects of trauma.
[0003]
By the way, due to the rapid development of molecular biology in recent years, genetic elements, that is, gene involvement in various diseases have been elucidated fairly accurately, and attention has been focused on gene-targeted medicine. Yes. At present, what is attracting the most attention is SNPs (snips). This is an abbreviation for single nucleotide polymorphism, which is generally translated as “single nucleotide polymorphism”, and is a general term for differences in one code (one base) in genes between individuals.
[0004]
All life-form genes on earth, including humans (or the genome that means the entire collection of genes), are composed of four common bases, and various proteins are created by the sequence of these bases. Life activities are taking place. The four bases common to all organisms are adenine (denoted as A), guanine (denoted as G), thymine (denoted as T), and cytosine (denoted as C). Human genes are said to be composed of about 3 to 3.2 billion base sequences, but each individual has a base that is different from other people at a rate of about one in several hundred to 1000 bases. Exists. Usually, this single base change is present at a frequency of 1% or more in the total population of a certain human population, and is called SNPs.
[0005]
Therefore, it is said that there are 3 to 10 million SNPs in all genes (genome), and the search for SNPs is currently continued all over the world. The reason why SNPs are attracting attention is that it is considered that the morbidity rate for many diseases, which are said to be statistically related to the genes of each individual, can be estimated by the classification of SNPs. For example, taking breast cancer as an example, SNPs common to those who are likely to have breast cancer can be identified by comparing SNPs between a group of patients with breast cancer and a normal group. At the time of a health examination, it becomes possible to find a person who has investigated the gene and has the SNPs, that is, a person who is normal but is likely to have breast cancer in the future.
[0006]
With this diagnosis, a person with a constitution that is likely to have breast cancer can be treated very early, and the possibility of survival can be improved even if he / she suffers from cancer. The same can be said for lifestyle-related diseases such as diabetes and hypertension, and it is possible to accurately diet and guide living before the onset of diseases that many people around the world suffer.
[0007]
In addition, SNPs are expected to play an important role regarding drugs used for treatment of diseases. Drugs used during treatment are not equally effective for everyone. In general, it is well known that drugs are effective for a certain proportion of people but not for others at all, and may cause adverse results due to side effects. Incidentally, it is well known that drug side effects are at the top of the causes of death in the United States. The effect of the drug is deeply related to the constitution of the person, and the constitution is said to be distinguishable by the classification of SNPs. That is, the classification based on the analysis of SNPs makes it possible to predict the effect and sensitivity of a certain drug in advance and make an appropriate prescription, and the optimal drug administration and risk of side effects according to the individual patient's constitution. Avoidance is expected. Such medical care is called tailor-made medical care or tailor-made medical care, and future practical use is surely expected.
[0008]
In addition, it is known that cancer is caused by a mutation occurring at a specific site on a gene that plays an important role in normal cells, for example, by the action of ultraviolet rays or mutagenic substances. By reading a mutation on a specific gene, it becomes possible to diagnose from an early stage whether or not a cell is cancerous. SNPs are also effective in identifying criminals in criminal investigations, determining ambiguous parent-child relationships, and identifying whether or not they are individuals. As described above, there are 3 to 10 million SNPs in each individual, and since there are separate SNPs from parents, there are absolutely no humans on the planet who have the same SNPs even if they are parents and siblings. It is said not to. This is the reason why complete identification of individuals is possible.
[0009]
In this manner, observing a mutation that occurs at one base in a specific gene may greatly contribute to various matters including medical treatment. However, at present, the method of observing a mutation of a specific gene requires a very complicated operation or an expensive apparatus as described below, and the running cost is very high, so that it has not yet been widely used. is there.
[0010]
The most commonly used method for examining SNPs at present is a method called sequencing (determining the base sequence) in which the base sequence of DNA is directly read from the end. Since a gene is a unit of DNA having base sequence information for forming one kind of protein, SNPs can be elucidated by reading the base sequence from the end. There are several reports on the sequencing method, but the most commonly performed method is dideoxy sequencing (Sanger method) described below. All of these methods, including this method, are based on a technique that can separate and identify the difference in length of one base length by denaturing polyacrylamide gel electrophoresis or capillary electrophoresis with high resolution.
[0011]
The dideoxy sequencing (Sanger method), also called enzymatic sequencing, uses DNA polymerase to synthesize complementary strands of single-stranded template DNA, and then produces four special types of dideoxynucleotides artificially created. The feature is to use. As a sequencing operation, a synthetic base sequence that complements the 3 'end of the single-stranded DNA to be sequenced is used as a primer, and deoxynucleotides added equally from the primer to DNA polymerase are extended by an enzymatic reaction. At this time, four reaction vessels were prepared at the same time, and each did not have a hydroxyl group at the 3 'end of the ATGC four bases, and therefore dideoxynucleotide, a base analog that could not continue the DNA extension reaction any more. Mix a small amount separately. As a result, DNA synthesis was stopped when dideoxynucleotide was added to the end of the extending DNA, and each reaction vessel had various lengths, but the ends were always added base analogs. Stranded DNA is formed. The reaction vessel is reacted with S1 endonuclease to digest all the single-stranded DNA into only double-stranded DNA. If the DNA strands of the four reaction vessels thus obtained are subjected to gel electrophoresis or capillary electrophoresis, and the separated DNA is read in order from the shorter one (moved faster), the base sequence of the DNA complementary to the template strand will be Recognize. At this time, the electrophoresis results are identified by, for example, radioactively labeling the added dideoxynucleotide phosphorus or sulfur or binding a fluorescent chemical substance. In the case of a radioactive label, detection is performed by exposure to a film. In the case of a fluorescent chemical substance, fluorescence is detected by irradiating a laser beam. Recently, a method has been developed in which four types of base analogs A, T, G, and C are labeled with four types of reagents having different fluorescence wavelengths, and the four colors of fluorescence are simultaneously detected.
[0012]
In this way, the conventional base sequence of a gene isolated and purified from a subject is determined by this dideoxy sequencing (Sanger method) or other base sequence determination method, and compared with a normal or standard base sequence. Confirmation of the presence of SNPs and mutations, identification of individuals, etc.
[0013]
[Problems to be solved by the invention]
As described above, genetic diagnosis and identification of individuals by gene using conventional gene sequencing methods are performed by isolating the target gene, then amplifying and purifying it, and using a device for determining the base sequence of the gene. Since it was performed by reading the base sequence of the target gene, the experiment required a huge amount of work, a very long time, and a great running cost. In addition, an automated apparatus for determining a base sequence is very expensive, occupies a large space, and requires a large amount of expensive reagents.
[0014]
Therefore, in order to solve such a conventional problem, the present invention can detect a genetic abnormality of one or more nucleotides in a short time, easily and accurately, and is small, light and inexpensive, and has a very low running cost. An object of the present invention is to provide a genetic diagnosis apparatus capable of automating diagnosis.
[0015]
Furthermore, an object of the present invention is to provide a genetic diagnosis method that can easily and accurately determine a gene abnormality of one or more nucleotides in a short time.
[0016]
[Means for Solving the Problems]
In order to solve the above problems, the genetic diagnosis apparatus of the present invention has a binding channel in which a first base sequence capable of hydrogen bonding to a DNA sample and a polymer compound are bound in a buffer channel in a buffer. A DNA conjugate for separation that separates a DNA sample into normal DNA and abnormal DNA from the difference between the second base sequence and the polymer compound, and the second base sequence is different from normal DNA and abnormal DNA. In addition, a delay DNA conjugate that distinguishes only noise DNA with an equivalent binding force and a DNA sample are filled, and by applying a constant voltage, the DNA in the sealed channel is electrophoresed, and the detection unit The amount of passage of normal DNA, abnormal DNA, and noise DNA is measured, respectively.
[0017]
Thereby, a genetic abnormality of one base or more can be detected easily and accurately in a short time, and the diagnosis can be automated with a small size, light weight, low cost, and very low running cost.
[0018]
In the genetic diagnosis method of the present invention, the first base sequence capable of hydrogen bonding to the DNA sample and the polymer compound are bound in the buffer solution in the sealed channel, and the DNA sample is determined from the difference in binding strength. Filled with a DNA conjugate for separation that separates normal DNA and abnormal DNA, followed by binding of the second base sequence and the polymer compound, and normal DNA and abnormal DNA to the second base sequence Fill with a delaying DNA conjugate that has equivalent binding force to distinguish only noise DNA, add a DNA sample, and then apply a positive potential to the second electrode and a negative potential to the first electrode, A predetermined constant voltage is applied between the second electrode and the first electrode, the DNA in the sealed channel is electrophoresed, normal DNA, abnormal DNA, and noise DNA are separated, normal DNA quantification or abnormal DNA Quantitative or The ratio of normal DNA and abnormal DNA, or, and detects the abnormal DNA.
[0019]
Thereby, even a single base difference gene abnormality can be detected easily and accurately in a short time, and the diagnosis can be automated at a low cost with a very low running cost.
[0020]
DETAILED DESCRIPTION OF THE INVENTION
The invention described in claim 1 includes a first container in which a buffer solution is stored and the first electrode is immersed, a second container in which the buffer solution is stored and the second electrode is immersed, a first container, and a second container. A sealed channel that is connected by filling a buffer containing a linear polymer and a DNA binding controller between the containers, a power supply unit that applies a positive potential to the second electrode and a negative potential to the first electrode, and a power supply unit A control unit that controls and applies a predetermined constant voltage between the second electrode and the first electrode, and a detection unit that is provided in the sealed channel and detects the amount of DNA passing through the interior, Is a DNA conjugate for separation in which a first base sequence capable of hydrogen bonding to a DNA sample and a polymer compound are bound in a buffer solution, and the DNA sample is separated into normal DNA and abnormal DNA from the difference in binding strength. And the second base sequence and the polymer compound are combined, and the second base sequence A DNA conjugate for delay that has only the same binding force to normal DNA and abnormal DNA and distinguishes only noise DNA, and a DNA sample are filled, and DNA in a closed channel is applied by applying a constant voltage. Is applied to the second electrode and the first electrode, so that a predetermined constant voltage is applied between the second electrode and the first electrode. However, since the DNA sample can be electrophoresed, the separation DNA conjugate and the delay DNA conjugate are combined with the polymer compound, so the migration speed is only a few percent compared to the DNA sample ( However, depending on the type and length of the polymer compound, it can be relatively fixed in a pseudo state. Thus, the DNA sample is electrophoretically passed through the retarding DNA conjugate and then the separating DNA conjugate portion. At that time, first, by using the difference in hydrogen bond strength with the DNA conjugate for delay, the migration speed of normal DNA and abnormal DNA group is reduced with respect to noise DNA, and further, the migration of normal DNA is performed with the DNA conjugate for separation. The speed can be reduced relative to the migration speed of abnormal DNA.
[0021]
Although there is affinity DNA as a method for delaying a DNA sample, it is common to fix affinity DNA on the wall surface of a closed channel such as a capillary tube, and the fixing process is difficult. However, according to the present invention, since it is pseudo-fixed, it is not necessary to make it disposable, and it is very easy to adjust the concentration of both conjugates and samples and the mixing ratio of both conjugates and samples. .
[0022]
While normal DNA and abnormal DNA move, they are first subjected to the action of the binding force of the delay DNA conjugate, and noise DNA that does not receive this action is migrated first when a voltage is applied and detected by the detector. The However, the binding force with the DNA conjugate for separation as well as the DNA conjugate for separation acts on the abnormal DNA (however, it is weaker by one base compared with normal DNA), and the action with the conjugate cannot be easily shaken off. Electrophoresis is performed later than the noise DNA, and is detected by the detection unit next to the noise DNA. The maximum binding force acts on normal DNA, and it migrates later than abnormal DNA as well as noise DNA, and is finally detected by the detection unit. Thereby, a difference can be caused in the detection time of the three DNAs.
[0023]
In this way, DNA and DNA can be separated in a short time of several minutes to tens of minutes because of the use of electrophoresis and DNA hydrogen bonding, and it is only necessary to apply a predetermined voltage, making it extremely easy to achieve an optimum voltage with high resolution. Therefore, it is possible to accurately detect the presence / absence of DNA abnormality, to be a small, lightweight, low running cost, and very easy to automate diagnosis.
[0024]
In the invention described in claim 2, the sealed flow path is filled with a buffer solution containing a linear polymer and a DNA binding control agent, and a separation DNA conjugate and a delay DNA conjugate are contained in the buffer solution. A separation sealed flow path cartridge filled in this order with a linear polymer in a separated state from a DNA sample, and having a separation section for mounting the separation closed flow path cartridge in a replaceable manner 2. The genetic diagnosis apparatus according to claim 1, wherein the separation sealing is preliminarily filled with a buffer solution containing a linear polymer and a DNA binding control agent, a separation DNA conjugate, a delay DNA conjugate, and a DNA sample. A flow path cartridge can be prepared, and it is only necessary to replace and attach the separation closed flow path cartridge to the separation section for each measurement, making measurement simple and easy It can be carried out.
[0025]
Since the invention described in claim 3 is the genetic diagnostic apparatus according to claim 1 or 2 characterized in that one or more sealed channels are provided, a delay DNA conjugate and The separation environment of normal DNA and abnormal DNA of the DNA sample can be changed for each sealed flow path by changing the separation DNA conjugate and the DNA binding control agent.
[0026]
The invention described in claim 4 is the genetic diagnosis apparatus according to any one of claims 1 to 3, characterized in that one or more types of DNA conjugates for delaying are included, so that the migration speed is delayed. It can be changed by changing the ratio of the DNA conjugate for use.
[0027]
The invention described in claim 5 is the genetic diagnosis apparatus according to any one of claims 1 to 4, wherein the DNA conjugate for separation and / or the DNA conjugate for delay is vinylated DNA. Therefore, it is possible to clearly separate normal DNA and abnormal DNA of a DNA sample for measurement.
[0028]
The invention described in claim 6 is characterized in that the normal DNA and the abnormal DNA are separated by adjusting the liquid in the closed flow path to 20 ° C to 60 ° C. Because it is a genetic diagnostic device, normal DNA and abnormal DNA can be bound to or detached from the DNA conjugate for separation and the DNA conjugate for delay by adjusting the temperature. Thereafter, each can be measured by the detection unit.
[0029]
The invention described in claim 7 is a fused silica capillary tube having an inner diameter of 50 to 100 μm. One of Therefore, the detection of abnormal DNA can be facilitated by detecting the amount of ultraviolet light passing therethrough.
[0030]
The invention described in claim 8 is characterized in that the closed flow path is a combination of a grooved plate and a plate that transmits 90% or more of ultraviolet rays. One of 6 Therefore, the detection of abnormal DNA can be facilitated by detecting the amount of ultraviolet light passing therethrough.
[0031]
The invention according to claim 9 is: Heating the closed channel; Separate the double helix DNA sample into a single-stranded DNA sample A high temperature part was provided. Claims 1 to 8 characterized in that One of Since it can be used as it is without performing the pretreatment which makes a DNA sample a single chain, it is possible to further automate the diagnosis.
[0032]
According to the tenth aspect of the present invention, the buffer solution is accommodated in the first container and the first electrode is immersed, the buffer solution is also accommodated in the second container and the second electrode is immersed, and the first container and the first container are immersed in the first container. Between the two containers, a buffer containing a linear polymer and a DNA binding control agent is filled and communicated through a sealed channel, and then the first base capable of hydrogen bonding to the DNA sample is placed in the buffer in the sealed channel. The sequence and polymer compound are combined, and a DNA conjugate for separation that separates the DNA sample into normal DNA and abnormal DNA from the difference in binding force is filled, and then the second base sequence and polymer compound are combined. Then, normal DNA and abnormal DNA are packed with a delay DNA conjugate that has an equivalent binding force to the second base sequence and discriminates only noise DNA, and further a DNA sample is added. Apply a positive potential to the electrode and A negative potential is applied to the electrode, a predetermined constant voltage is applied between the second electrode and the first electrode, the DNA in the sealed channel is electrophoresed, and normal DNA, abnormal DNA, and noise DNA are separated, Since it is a genetic diagnosis method characterized by detecting normal DNA quantification or abnormal DNA quantification, or the ratio of normal DNA to abnormal DNA, or abnormal DNA, a predetermined amount between the second electrode and the first electrode A DNA sample can be electrophoresed by applying a constant voltage. However, since the separation DNA conjugate and the delay DNA conjugate are combined with a polymer compound, the migration speed is several percent compared to the DNA sample. However, it depends on the type and length of the polymer compound, and can be relatively fixed in a pseudo state. Thus, the DNA sample is electrophoretically passed through the retarding DNA conjugate and then the separating DNA conjugate portion. At that time, first, by using the difference in hydrogen bond strength with the DNA conjugate for delay, the migration speed of normal DNA and abnormal DNA group is reduced with respect to noise DNA, and further, the migration of normal DNA is performed with the DNA conjugate for separation. The speed can be reduced relative to the migration speed of abnormal DNA.
[0033]
Although there is affinity DNA as a method for delaying a DNA sample, it is common to fix affinity DNA on the wall surface of a closed channel such as a capillary tube, and the fixing process is difficult. However, according to the present invention, since it is pseudo-fixed, it is not necessary to make it disposable, and it is very easy to adjust the concentration of both conjugates and samples and the mixing ratio of both conjugates and samples. .
[0034]
While normal DNA and abnormal DNA move, they are first subjected to the action of the binding force of the delay DNA conjugate, and noise DNA that does not receive this action is migrated first when a voltage is applied and detected by the detector. The However, the binding force with the DNA conjugate for separation as well as the DNA conjugate for separation acts on the abnormal DNA (however, it is weaker by one base compared with normal DNA), and the action with the conjugate cannot be easily shaken off. Electrophoresis is performed later than the noise DNA, and is detected by the detection unit next to the noise DNA. The maximum binding force acts on normal DNA, and it migrates later than abnormal DNA as well as noise DNA, and is finally detected by the detection unit. Thereby, a difference can be caused in the detection time of the three DNAs.
[0035]
In this way, DNA and DNA can be separated in a short time of several minutes to tens of minutes because of the use of electrophoresis and DNA hydrogen bonding, and it is only necessary to apply a predetermined voltage, making it extremely easy to achieve an optimum voltage with high resolution. The presence or absence of DNA abnormality can be accurately detected.
[0036]
Hereinafter, a genetic diagnostic apparatus and a genetic diagnostic method according to embodiments of the present invention will be described with reference to the drawings.
[0037]
(Embodiment 1)
FIG. 1 is an external view of a genetic diagnostic apparatus according to Embodiment 1 of the present invention, FIG. 2 is an external view of the genetic diagnostic apparatus according to Embodiment 1 of the present invention, and FIG. 3 is a gene according to Embodiment 1 of the present invention. FIG. 4 is a main part diagram of the control circuit of the genetic diagnosis apparatus according to the first embodiment of the present invention, and FIG. 5 is a diagram for separation in the sealed flow path of the genetic diagnosis apparatus according to the first embodiment of the present invention. It is an introduction state figure of a DNA conjugate, a DNA conjugate for delay, and a DNA sample.
[0038]
In FIG. 1, 1 is a power switch of the genetic diagnosis apparatus, 2 is an operation button for performing various operations of the apparatus, 3 is a display panel, 4 is an upper lid, and 5 is a casing of the apparatus. 2, 3, and 4, 6 is an electrophoresis unit for performing electrophoresis, 7 is a support base that supports the electrophoresis unit 6, 8 is a control for performing electrophoresis, a suction pump 20 described later, and detection. It is a control calculation part which consists of a board | substrate which controls the part 15 and calculates the detected data. Reference numeral 9 denotes a power supply box, and 9a denotes a power supply unit provided in the power supply box 9. The power supply unit 9a is most suitable for separating abnormal DNA and normal DNA from a DNA sample 23, which will be described later, because there is an optimum applied voltage value that differs depending on the type, concentration, and processing conditions of DNA in this genetic diagnosis apparatus. A predetermined voltage is applied under the control of the control calculation unit 8 so that electrophoresis can be performed. 10 is a high temperature part for separating the double helix (hereinafter, double strand) of DNA, 11 is a heat insulating part for making the temperature of the high temperature part 10 and the separation part 12 described later independent, and 12 is normal DNA and abnormal DNA And a separation unit that separates normal DNA and abnormal DNA in this part, 13 is a first temperature controller that regulates the temperature of the high temperature part 10, and 14 is a separation part. It is the 2nd temperature controller which adjusts the temperature of 12.
[0039]
The details of the configuration in the separation unit 12 will be described later. At the start of measurement, as shown in FIG. 5, the separation DNA conjugate 21 is located at the separation unit 12, and the delay DNA conjugate 22 is near the heat insulation unit 11. The DNA sample 23 is arranged so as to be in the vicinity of the high temperature part 10. Then, by performing the arrangement, voltage control, concentration adjustment, temperature control, and the like set in this way, the present gene diagnosis apparatus converts the DNA sample 23 into normal DNA, abnormal DNA, and noise DNA for several minutes to 10 minutes while performing electrophoresis. It will separate in minutes.
[0040]
Among them, the DNA sample 23 is filled and arranged in the high temperature part 10 with double strands in the first embodiment, and the first temperature controller 13 is used (predetermined temperature of 90 ° C. or higher ± 5 ° C.). It is heated and controlled so that the temperature becomes. The double strands of DNA introduced by this heating are automatically separated into single strands. Subsequently, in the separation unit 12, the DNA sample 23 is abnormally treated as normal DNA due to a difference in hydrogen bonding strength while the separation DNA conjugate 21 (and in some cases, some of the retardation DNA conjugates 22) is subjected to an electrophoretic action. In order to be able to separate DNA from noise DNA, the temperature is controlled to be at least 10 ° C. lower than the temperature of the high temperature portion 10, that is, at a predetermined temperature in the temperature range of 15 ° C. to 80 ° C., preferably 20 ° C. to 60 ° C. In order to separate normal DNA from abnormal DNA, it is preferable to control within a range of ± 1 ° C. from this predetermined temperature suitable for DNA separation. Further, the heat insulating part 11 is originally provided to adjust the temperature by thermally blocking between the separating part 12 and the high temperature part 10, but the delaying DNA conjugate 22 is disposed in the vicinity thereof, In terms of temperature, it is placed at an intermediate temperature between the temperature of 90 ° or higher of the high temperature part 10 and the temperature of 20 ° C. to 60 ° C. of the separation part 12, while undergoing the electrophoretic action due to the difference in hydrogen bond strength at this temperature. Normal DNA and abnormal DNA can be separated from noise DNA.
[0041]
Reference numeral 15 denotes a detection unit that measures the passing amount of the DNA sample to be electrophoresed. The detection unit 15 will be described with reference to FIG. ₂ A lamp, 15b is a photodiode that receives ultraviolet light, 15c is a preamplifier that amplifies a weak current detected by the photodiode 15b, and 15d is an A / D converter that converts it into a digital quantity. Details of these will be described later. Reference numeral 16 denotes an electrode that applies a positive potential during electrophoresis (second electrode of the present invention), and 17 denotes an electrode that applies a negative potential during electrophoresis (first electrode of the present invention). Controls the power supply unit 9a and applies a predetermined constant voltage between the electrode 16 and the electrode 17 to cause the most appropriate electrophoresis. 3, 4, and 5, 18 is a buffer solution for carrying charge during electrophoresis and stabilizing the pH of the DNA sample, and 18 a is a cathode-side container containing the buffer solution 18 (the first embodiment of the present invention). 1 container), 18b is a container on the anode side (second container of the present invention) containing the buffer solution 18, and 18d is a linear polymer gel in which a DNA binding control agent and a linear polymer are added to the buffer solution 18. The DNA sample 23 has a function of hindering migration so that it does not migrate at a high speed. This function makes it possible for the DNA sample 23 to have sufficient opportunity to encounter the delay DNA conjugate 22 or the separation DNA conjugate 21 in the capillary tube 19. Reference numeral 19 denotes a capillary tube (a sealed channel of the present invention) for electrophoresis of the DNA sample 23 during electrophoresis, and 20 denotes a buffer solution 18, a DNA sample 23, a linear polymer gel 18 d, etc. in the capillary tube 19. A suction pump for injecting a reagent. The electrode 17 is immersed in the buffer solution 18 of the container 18a, and the electrode 16 is immersed in the buffer solution 18 of the container 18b. The buffer 18 in the container 18a and the container 18b is communicated with the buffer 18 in the capillary tube 19. Therefore, the buffer solution 18 is mixed as a base of the solution into the separation DNA conjugate 21 and the delay DNA conjugate 22, and the buffer solution 18 having the same concentration exists in all portions in the capillary tube 19. When a voltage is applied between the electrode 16 and the electrode 17, electrophoresis is induced in the capillary tube 19, and the separation DNA conjugate 21, the delaying DNA conjugate 22, and the DNA sample 23 are negatively charged. The separation DNA conjugate 21, the delay DNA conjugate 22, and the DNA sample 23 move from the 18a side to the container 18b side. The separation DNA conjugate 21 and the delay DNA conjugate 22 have a high molecular weight. Therefore, there is almost no movement compared to the movement amount of the DNA sample 23 by electrophoresis.
[0042]
Next, details necessary for performing measurement with the genetic diagnosis apparatus of the present invention will be described. The DNA sample 23 measured by this genetic diagnostic apparatus is DNA obtained from human cells, blood, or the like. It is necessary to cut out the target portion from the human genomic DNA, which is said to have about 3 billion base pairs, to a target length using a method such as PCR (polymerase chain reaction) and increase the number for measurement. However, since this PCR is not necessary for the description of the present gene diagnostic apparatus, a specific description is omitted.
[0043]
The target DNA extracted by PCR or the like is about 6 to 1000 in terms of the number of bases, but it is probable that the same DNA sequence does not exist in human genomic DNA which is said to have about 3 billion base pairs. The number considered is about 50. However, this means that the total number should be about 50. Therefore, when the DNA is cut out in several times, it may be divided into 6 to 12 pieces. According to the experiments of the present inventors, when separating normal DNA and abnormal DNA having one base difference with this genetic diagnosis apparatus, the result is that the number of bases can be separated most efficiently from 6 to 12. Yes. However, the abnormal DNA is separated by the concentration of the DNA sample 23 (μM, where M = mol / liter), the concentration of the DNA of the separating DNA conjugate 21 (mol%), and the concentration of the DNA of the delaying DNA conjugate 22. (Mole%), measurement temperature, and other factors have a close relationship with each other, and separation does not occur unless appropriate conditions are used. It is necessary to pay attention to whether such conditions can be set. For example, the concentration of the DNA sample 23 is suitably 1 to 10 (μM), and the DNA contained in the separation DNA conjugate 21 and the delaying DNA conjugate 22 has a concentration of 0.1 to the molar amount of the basic linear polymer. Although about 0002 to 0.05 (mol%) is appropriate, the total DNA amount of the separation DNA conjugate 21 and the delaying DNA conjugate 22 should be 20 to 600 times the concentration of the DNA sample 23. desirable. As described above, the DNA sample of this genetic diagnostic apparatus requires a DNA sample having a base sequence of about 6 to about 1000 obtained by pretreatment by the above-described PCR or the like, and appropriate conditions must be set. .
[0044]
Next, the capillary tube 19 shown in FIGS. 3, 4 and 5 will be described. When a gel is placed in the capillary tube 19 and electrophoresis is performed, a liquid flow called electroosmotic flow is generated. It is necessary to prevent this phenomenon from occurring in the diagnostic apparatus. For this reason, it is preferable to coat the inner wall of the capillary tube 19 with acrylamide or the like. As long as the generation of the electroosmotic flow can be prevented, another coating method may be used. For example, a commercially available coated capillary tube may be used. As the capillary tube 19, a fused silica capillary tube having an inner diameter of 50 to 100 μm can transmit ultraviolet rays of 90% or more, and when DNA is detected using ultraviolet rays as will be described later, the amount of passing ultraviolet rays is easy. It is most suitable because it can be detected. Further, even if a closed channel corresponding to the capillary tube 19 is configured by a combination of a plate with a groove and a plate that transmits 90% or more of ultraviolet rays, it can transmit 90% or more of ultraviolet rays and detect the amount of passing ultraviolet rays. Thus, abnormal DNA can be easily detected. When the grooved plate is made a plate that can transmit ultraviolet rays, transmitted light is detected. When the grooved plate is made a plate that does not transmit ultraviolet rays, abnormal DNA is detected by reflected light. When detecting the reflected light, it is necessary to devise a rectangular cross section to make the groove shape a uniform reflecting surface.
[0045]
As the buffer solution 18 accommodated in the containers 18a and 18b or the capillary tube 19, it is appropriate to use a Tris-Borate (pH 7.2 to pH 8) buffer solution or the like. Among these, as a DNA binding control agent mixed as necessary in the buffer solution 18 accommodated in the capillary tube 19, magnesium chloride or the like that promotes DNA binding to the separation DNA conjugate 21 or the delaying DNA conjugate 22 is used. There are two types: binding promoters and release agents such as urea that promote release. These two types of DNA binding control agents can control various migration speeds for DNA by selecting two types of mixing ratios and substances (for example, other electrolytes as binding promoters). As the linear polymer contained in the linear polymer gel 18d, polyacrylamide can be used. Since this is also used for the preparation of the conjugate of the separation DNA conjugate 21 and the delaying DNA conjugate 22, the compatibility is good and appropriate. It is.
[0046]
Next, the order of filling the capillary tube 19 is as follows. First, as shown in FIG. 5, a linear polymer gel 18d containing a linear polymer, a DNA binding control agent and a buffer solution 18 is introduced into the capillary tube 19, and then Add the DNA conjugate for separation 21 detailed below. The linear polymer gel 18d may be introduced after the DNA conjugate 21 for separation is introduced. In the case of FIG. 5, it is introduced in a separated state after introduction. Subsequently, the DNA conjugate for separation 21 and the DNA conjugate for delay 22 are added in a separated state. Similarly to the separation DNA conjugate 21, the linear polymer gel 18d may be introduced after the introduction of the retardation DNA conjugate 22. In the case of FIG. 5, it is introduced in a separated state after introduction. Thereafter, DNA sample 23 diluted with buffer 18 or pure water is introduced and electrophoresed.
[0047]
In the first embodiment, since acrylamide and DNA are polymerized to produce the separation DNA conjugate 21 and the delay DNA conjugate 22, the weight difference and the structure difference from the DNA are large, and the separation DNA conjugate. The migration speed of the gate 21 and the delay DNA conjugate 22 (0.6 cm / min to 0.7 cm / min) is 1/20 to 1/30 of the optimal DNA migration speed (13 cm / min to 20 cm / min). A state is realized in which the movement is very slow and it may be said that it is relatively fixed in a pseudo manner. Therefore, at the start of measurement, the capillary tube 19 containing the packing is adjusted between the high temperature part 10, the heat insulation part 11 and the separation part 12, while the separation DNA conjugate 21 is placed in the vicinity of the separation part 12 to insulate the capillary tube 19. A delaying DNA conjugate 22 is placed from the vicinity of the portion 11 to the high temperature portion 10, and a DNA sample 23 described later is placed in the high temperature portion 10. By doing so, the double strands of the DNA sample 23 can be separated into single strands in the high temperature part 10. Since the delay DNA conjugate 22 is filled from the high temperature part 10 to the heat insulation part 11, noise DNA can be separated by a speed difference, and normal DNA and abnormal DNA can be separated by the separation part 12.
[0048]
In addition, a mechanism for exchanging DNA sample 23, DNA conjugate for separation, DNA conjugate for delay, and linear polymer into the capillary tube 19 of the genetic diagnosis apparatus, such as the suction pump 20 shown in FIG. In addition, a container for storing each solution of each DNA sample 23, DNA conjugate for separation, DNA conjugate for delay, and linear polymer, and a mechanism for automatically exchanging the container and connecting it to the capillary tube 19 are provided. It is desirable to equip.
[0049]
Furthermore, the capillary tube 19 is unitized in units of one or a plurality of units, and this can be attached to the separation unit 12, the high temperature unit 10, and the heat insulation unit 11 as a separation sealed channel cartridge for replacement. It is also appropriate to control the temperature with the second temperature controller 14 or the first temperature controller 13 in the high temperature part 10. The capillary tube 19 is previously filled with a linear polymer gel 18d and a buffer solution 18 containing a DNA binding control agent, and the separation DNA conjugate 21, the delaying DNA conjugate 22 and the DNA sample 23 are filled in a separated state and separated. It becomes possible to prepare as a closed flow path cartridge for use. With this configuration, each separation sealed flow path cartridge is replaced every time measurement is performed. Therefore, the separation DNA conjugate 21, the delay DNA conjugate 22, and the DNA sample 23 are separated for each separation sealed flow path cartridge. Since the arrangement can be set in advance, the measurement can be performed easily and accurately. In this separation sealed flow path cartridge, the separation DNA conjugate 21, the delay DNA conjugate 22 and the DNA sample 23 are separated and filled with a linear polymer gel 18d therebetween. The linear polymer gel 18d may be mixed and filled in each of them.
[0050]
Next, the separation DNA conjugate 21 and the delay DNA conjugate 22 will be described. FIG. 6 (a) is a conceptual diagram of the relationship between the DNA conjugate for separation and the DNA sample in the closed flow path of the genetic diagnosis apparatus according to the first embodiment of the present invention, and FIG. 6 (b) is the first embodiment of the present invention. It is a conceptual diagram of the relationship between the DNA conjugate for delay and the DNA sample in the closed flow path of the genetic diagnosis apparatus in FIG. 6 (a) and 6 (b), 21 is a DNA conjugate for separation, and 22 is a DNA conjugate for delay. There are two types of DNA: one that forms a double strand and one that separates the DNA, but the four bases A, T, C, and G of DNA have hydrogen bonds A and T and G and C, respectively. It has an easy property, and the double strand of DNA is paired with AT and GC. Therefore, when the single-stranded DNA is arranged as ATCGCGTCTAGC (described in SEQ ID NO: 1), the remaining DNA has a base sequence of TAGCGCAGATCG (described in SEQ ID NO: 2). This relationship is called a complementary relationship. As long as this complementary relationship is satisfied, A and T and G and C are bonded by hydrogen bonds to form a double strand. In the present invention, in order to utilize this relationship, as shown in FIG. 6A, the DNA portion of the separating DNA conjugate 21 has a base sequence complementary to the normal DNA of the DNA sample. Therefore, the normal DNA base sequence of the DNA sample contains ATCGCGTCTAGC (described in SEQ ID NO: 1), and the abnormal DNA is ATCA. ^* In CGTTAGAGC (described in SEQ ID NO: 3), when the bases of normal DNA and abnormal DNA are different in the part indicated by *, the DNA part sequence of the DNA conjugate for separation 21 (first base sequence of the present invention) Is TAGCGCAGATCG (described in SEQ ID NO: 2), the abnormal DNA is A ^* In FIG. 2, hydrogen bonds do not occur because they are no longer complementary to the separation DNA conjugate 21, and the binding force of the entire hydrogen bond is larger by the binding force of one base than the abnormal DNA in the normal DNA of the DNA sample. As a result, during electrophoresis described later, normal DNA binds to separation DNA conjugate 21 for a longer time with a stronger binding force than abnormal DNA, so normal DNA is delayed relatively than abnormal DNA. This is because not only the binding force during electrophoresis but also the pulling force due to electrophoresis acts, so that a large number of DNAs are in a binding state that repeats binding and detachment intermittently. When this migration speed is viewed on average, the migration speed of normal DNA that binds for a long time is lower than that of abnormal DNA. The DNA sample includes DNAs other than normal DNA and abnormal DNA, such as the remaining separated single-stranded DNA that is not the target of measurement, out of double-stranded DNA, and this DNA will be described later. Although it acts as noise during electrophoresis, the noise DNA is hardly reacted with the DNA of the DNA conjugate for separation 21 and binds with the fastest migration speed.
[0051]
In order to reliably separate the noise DNA from the group of normal DNA and abnormal DNA in advance, a base sequence complementary to the base sequence common to both normal DNA and abnormal DNA in the delay DNA conjugate 22 (the present invention). 2), only the normal DNA group and the abnormal DNA group hydrogen bond with the delay DNA conjugate 22 during electrophoresis, and the migration speed is lower than that of the noise DNA. Therefore, the group of normal DNA and abnormal DNA is relatively delayed from the noise DNA, and it becomes possible to distinguish the noise DNA and eliminate its influence. Noise DNA is bound by chance when a base is hydrogen-bonded by chance, which is very low stochastically. Note that the base sequence of the delay DNA conjugate 22 (second base sequence of the present invention) is normal because both normal DNA and abnormal DNA are hydrogen-bonded to the delay DNA conjugate 22 and separated from the noise DNA. It must be complementary to the base sequence possessed by both DNA and abnormal DNA, and is preferably, for example, GCAGATCG (described in SEQ ID NO: 4) as shown in FIG. In order to select a base sequence that can be reliably bound only to normal DNA and abnormal DNA, the base sequence should be long in order to increase the probability of binding only to both. The total DNA amount of the delay DNA conjugate 22 and the separation DNA conjugate 21 is suitably 20 to 600 times the concentration of the DNA sample.
[0052]
Next, a method for producing and synthesizing such a separation DNA conjugate 21 and a delaying DNA conjugate 22 will be described. In order to synthesize vinylated DNA, DNA for separation DNA conjugate 21 and delay DNA conjugate 22 is cut out by PCR. In the above-described example, TAGCGCAGATCG (described in SEQ ID NO: 2) is the DNA of the separation DNA conjugate 21, and GCAGATCG (described in SEQ ID NO: 4) is the DNA of the delay DNA conjugate 22.
[0053]
Next, the 5 ′ end of the DNA having the desired base sequence is aminated (usually aminated via a hexyl group). The aminated DNA thus obtained is diluted by adding ultrapure water sterilized to 2.6 mM. Next, MOSU (methacryloid oxysuccinimide) is diluted with DMSO (dimethyl sulfoxide) to 71.388 mM. Then, the aminated DNA thus obtained and MOSU are added and adjusted so as to have a ratio of 1:50. Further, a solution adjusted with sodium hydrogen carbonate and sodium hydroxide so as to have a pH of 9 for pH adjustment is added to this adjusted solution in an amount equal to the amount of aminated DNA.
[0054]
The resulting solution is then shaken overnight. Thereafter, the vinylated DNA in the shaken solution is separated from the aminated DNA, MOSU, and others using HPLC (High Performance Liquid Chromatography). Since vinylated DNA contains an eluent (TEAA; mixed solution of triethylamine-acetic acid and acetonitrile), it is further concentrated under reduced pressure by a centrifugal evaporator having a vacuum drying function.
[0055]
Then, 53 μmol of nitrogen is substituted for 10% AAM (acrylamide) as a polymerization solution. Further, 1.34% of TEMD (N, N, N′N′-tetramethylethylenediamine) which is a polymerization initiator is diluted with sterilized ultrapure water deaerated by ultrasonic waves. This is diluted with sterilized ultrapure water in which 1.34% APS (ammonium persulfate), which is a polymerization initiator, is similarly degassed by ultrasonic waves. Furthermore, the concentrated vinylated DNA is diluted with sterilized ultrapure water. Then, in order to synthesize 100 μl of DNA conjugate, 34 μl of the above AAM, 5 μl each of the above TEMD and APS, and 0.01% to 0.05% mol of vinylated DNA with respect to AAM In addition, sterilized ultrapure water is added to 100 μl and left for about 60 minutes to obtain an acrylamideated DNA conjugate.
[0056]
In addition, in order to remove the unreacted vinylated DNA, a DNA conjugate having a high purity can be obtained by performing gel filtration with an appropriate pore size selected in several tens of times. In the first embodiment, the synthesis method is the same between the separation DNA conjugate 21 and the delay DNA conjugate 22, but different synthesis methods can be used.
[0057]
Subsequently, the operation of the genetic diagnosis apparatus according to the first embodiment will be described. First, a capillary tube 19 into which a DNA sample or each solution has been introduced is set in the genetic diagnosis apparatus, and the buffer solution 18 in the containers 18a and 18b is immersed at both ends as shown in FIGS. A predetermined voltage described later is applied between the electrode 16 and the electrode 17 by the power supply unit 9a. The appropriate voltage width is preferably 10 to 20 kilovolts, but may be 100 to 30 kilovolts depending on the state of the electrolyte and electrodes. For example, when the electrolyte concentration is low or the electrode area is large, the voltage is lowered. Then, instead of applying a predetermined voltage from the beginning, if a high voltage of 30 kilovolts or more for preparation is applied before applying a constant voltage and noise DNA is quickly separated, the measurement can be performed quickly.
[0058]
Here, the reason why the predetermined voltage is applied will be explained. The difference between the binding force of the DNA sample to the delaying DNA conjugate 22 and the separating DNA conjugate 21 and the separation force due to the electrophoretic force is the migration of DNA. This is because it has a great influence on the speed and movement difference, and it is necessary to perform electrophoresis by applying a predetermined constant voltage at which separation of normal DNA, abnormal DNA and noise DNA is most effectively performed. That is, this voltage must be as low as possible in order to increase the resolution, since the normal DNA that is most difficult to migrate can be electrophoresed, and the resolution of normal DNA and abnormal DNA decreases when high voltage is applied. The voltage satisfies the two conditions. Accordingly, an optimum voltage to be applied in advance is examined for each DNA and for each condition, and after initially applying a preparation voltage of about 30 kilovolts or more for a short time, this voltage is applied. Since the DNA in the capillary tube 19 is negatively charged and proceeds to the anode side, the power supply unit 9a needs to apply the electrode 16 so as to have a positive potential and the electrode 17 have a negative potential. In addition, in electrophoresis, if the migration time is too long, the buffer solution 18 is dried in the capillary tube 19, so it is necessary to avoid running for a longer time than necessary.
[0059]
When a voltage is applied, the DNA sample migrates, and the normal DNA group and the abnormal DNA group have the same binding strength with the DNA conjugate 22 for delay, and thus migrate in exactly the same way while repeating intermittent binding and detachment. Therefore, a large movement difference occurs between the noise DNA and the group of normal DNA and abnormal DNA. The separation DNA conjugate 21 has a difference of one base in the binding force between normal DNA and abnormal DNA. When the DNA conjugate 21 is migrated, a difference in movement speed occurs between the two, and a difference in movement occurs between the two.
[0060]
Next, the high temperature part 10 where the separation is performed, the separation part 12, and the heat insulating part 11 will be described. As described above, in order to release the double strands of DNA in the high temperature part 10, the temperature is controlled using the first temperature controller 13 so that the temperature becomes 90 ° C. or higher (predetermined temperature ± 5 ° C.). In the separation unit 12, although depending on the state of the DNA sample, normal DNA, abnormal DNA, or noise DNA is determined based on the difference in binding force between the separation DNA conjugate 21 or the delay DNA conjugate 22 and the DNA sample. Must be kept at a predetermined temperature in the temperature range of about 15 ° C. to 80 ° C., preferably 20 ° C. to 60 ° C., about 10 ° C. lower than the temperature of the high temperature section 10. In the genetic diagnosis apparatus of the first embodiment, a silicon rubber heater, a nichrome wire, etc., and a temperature sensor such as a thermocouple, thermal, etc. are disposed below the separation unit 12 covering the capillary tube 19, and the second temperature controller 14. The temperature is controlled to be a predetermined temperature ± 1 ° C. or less. However, depending on the environmental temperature, the room temperature may exceed the target predetermined temperature, and it is better to use a component that can be heated and cooled such as Peltier instead of a silicon rubber heater or nichrome wire. Further, the heat insulating part 11 may be made of a heat insulating material such as glass wool, a foaming agent, mica, porous ceramics or the like whose contents are evacuated. In the vicinity of the heat insulating portion 11, the delaying DNA conjugate 22 has an intermediate temperature between the high temperature portion 10 and the separation portion 12, and thus normal DNA and abnormal DNA can be separated from noise DNA.
[0061]
Next, how to detect normal DNA, abnormal DNA, and noise DNA in which the migration speed is different due to the action of the delay DNA conjugate 22 and the separation DNA conjugate 21 and the migration difference is generated will be described. . FIG. 7 is a graph showing the relationship between the elapsed time and the absorbance when the elapsed time from the start of electrophoresis is plotted on the horizontal axis and the absorbance is plotted on the vertical axis. The detection is performed by measuring the absorbance when ultraviolet irradiation is shielded by normal DNA, abnormal DNA, and noise DNA. In the first embodiment, as shown in FIG. 5, the glass portion is exposed at a part of the capillary tube 19, and D ₂ An ultraviolet ray having a wavelength of 260 nm is irradiated from the lamp 15a, and the ultraviolet irradiation light obtained at this time is detected by a photodiode 15b, and the absorbance is measured. The control operation unit 8 controls the power supply unit 9a to ₂ The current detected by the photodiode 15b by causing the lamp 15a to emit light is amplified by the preamplifier 15c, and converted into the absorbance as a digital amount by the A / D converter 15d by the control calculation unit 8. The control calculation unit 8 has a built-in timer (not shown), and can measure the elapsed time from the migration start time. In FIG. 7, the earliest in time (I) is the noise DNA that does not bind to the DNA conjugate, the middle time (II) is abnormal DNA, and the late time (III) is normal DNA.
[0062]
From this relationship diagram, if the peak height, time, and number of peaks are read, it can be seen from the number of peaks that the DNA sample contains abnormal DNA. That is, it can be determined from the number of peaks whether abnormal DNA exists. Since the number of peaks can be limited to abnormal DNA and noise DNA depending on the applied voltage, DNA concentration, and DNA length (number of bases), only the passing amount of abnormal DNA is measured at this time. In addition, comparing peak heights shows the difference in absorbance between two groups with different migration speeds in DNA electrophoresed under the same conditions, which corresponds to the abundance ratio of abnormal DNA and normal DNA. The ratio can be determined. To determine the abundance of abnormal DNA, standard data obtained from the detection peak waveform of a standard DNA sample may be input in advance to the control calculation unit 8, and the data may be compared with the measured data for conversion.
[0063]
As described above, according to the genetic diagnosis apparatus and the genetic diagnosis method of the first embodiment, among DNA extracted from cells, blood, etc., a specific DNA is included in a DNA sample extracted with a restriction enzyme or the like. By knowing the abundance ratio of normal DNA and abnormal DNA to be detected, genetic diagnosis and determination can be made.
[0064]
(Embodiment 2)
A genetic diagnostic apparatus and a genetic diagnostic method according to Embodiment 2 of the present invention will be described with reference to FIGS. 1, 2, and 4 to 8. FIG. 8 is an apparatus configuration diagram of the genetic diagnosis apparatus according to the second embodiment of the present invention. The genetic diagnostic apparatus of the second embodiment corresponds to the single-stranded DNA of the DNA diagnostic apparatus of the first embodiment as a DNA sample and is basically the same as the genetic diagnostic apparatus of the first embodiment. Therefore, only the characteristic part will be described, and the detailed description will be omitted to the first embodiment.
[0065]
As shown in FIG. 8, in the genetic diagnosis apparatus of the second embodiment, the separation DNA conjugate 21, the delay DNA conjugate 22, and the single-stranded DNA sample 23 are directly introduced into the separation unit 12. That is, the electrophoresis unit 6 is basically composed of only the separation unit 12. The high temperature part 10 and the heat insulation part 11 of Embodiment 1 do not exist. In the case of introduction in the form of a separation sealed flow path cartridge, the capillary tube 19 filled with the separation DNA conjugate 21, the delaying DNA conjugate 22 and the DNA sample 23 in this order is replaced and separated for each measurement. Attach to part 12.
[0066]
In the first embodiment, a double-stranded DNA sample 23 is supplied, and a high-temperature unit 10 is provided to automatically make this a single-stranded DNA. However, in the second embodiment, the single-stranded DNA is supplied as the DNA sample 23 and there is no need to separate the double-stranded DNA, so that the high temperature part 10 and the heat insulating part 11 are not required. . Therefore, at the start of measurement, if the separation DNA conjugate 21 and the delay DNA conjugate 22 are arranged in the vicinity of the separation unit 12 and the DNA sample 23 is in the vicinity of the entrance of the separation unit 12, the measurement can be immediately executed. And the 2nd temperature controller 14 of the isolation | separation part 12 is controlled so that it may maintain at the predetermined temperature of 15 to 80 degreeC similarly to Embodiment 1, desirably 20 to 60 degreeC. By controlling the temperature in this manner, the DNA sample 23 can be separated into normal DNA, abnormal DNA, and noise DNA by the separation DNA conjugate 21 and the delay DNA conjugate 22.
[0067]
Thus, since the genetic diagnostic apparatus of Embodiment 2 does not require the high temperature part 10 and the heat insulating part 11, the configuration of the diagnostic apparatus can be simplified, can be easily controlled, and can be handled easily.
[0068]
【The invention's effect】
As described above, according to the present invention, the following advantageous effects can be obtained.
[0069]
In the genetic diagnostic apparatus according to claim 1, although a predetermined constant voltage is applied between the second electrode and the first electrode and the DNA sample can be electrophoresed, the DNA conjugate for separation, the DNA conjugate for delay Since the gate is bound to the polymer compound, the migration speed is only a few percent compared to the DNA sample (however, it depends on the type and length of the polymer compound), and is relatively in a pseudo-fixed state. can do. Thus, the DNA sample is electrophoretically passed through the retarding DNA conjugate and then the separating DNA conjugate portion. At that time, first, by using the difference in hydrogen bond strength with the DNA conjugate for delay, the migration speed of normal DNA and abnormal DNA group is reduced with respect to noise DNA, and further, the migration of normal DNA is performed with the DNA conjugate for separation. The speed can be reduced relative to the migration speed of abnormal DNA.
[0070]
Although there is affinity DNA as a method for delaying a DNA sample, it is common to fix affinity DNA on the wall surface of a closed channel such as a capillary tube, and the fixing process is difficult. However, according to the present invention, since it is pseudo-fixed, it is not necessary to make it disposable, and it is very easy to adjust the concentration of both conjugates and samples and the mixing ratio of both conjugates and samples. .
[0071]
While normal DNA and abnormal DNA move, they are first subjected to the action of the binding force of the delay DNA conjugate, and noise DNA that does not receive this action is migrated first when a voltage is applied and detected by the detector. The However, the binding force with the DNA conjugate for separation as well as the DNA conjugate for separation acts on the abnormal DNA (however, it is weaker by one base compared with normal DNA), and the action with the conjugate cannot be easily shaken off. Electrophoresis is performed later than the noise DNA, and is detected by the detection unit next to the noise DNA. The maximum binding force acts on normal DNA, and it migrates later than abnormal DNA as well as noise DNA, and is finally detected by the detection unit. Thereby, a difference can be caused in the detection time of the three DNAs. Since electrophoresis and DNA hydrogen bonding are used, DNA can be separated in a short time of several minutes to several tens of minutes, and it is only necessary to apply a predetermined voltage, so it can be adjusted very easily to an optimum voltage with high resolution. Therefore, it is possible to accurately detect the presence or absence of DNA abnormality, and to make the device small, light, and low in running cost, and it is extremely easy to automate diagnosis. As a result, with respect to diseases caused by mutations in various genes such as cancer, diabetes, hypertension, and Alzheimer, it is possible to predict the risk of onset for the disease and prevent it before onset or detect it at an extremely early stage. In addition, by investigating the diversity of genes possessed by each individual, it becomes possible to presume in advance the presence or absence of side effects and effects of the drug, and to provide a drug most suitable for each individual. Furthermore, it is possible to quickly determine and use gene mutations collected from tissues that have undergone mutation and have become cancerous. The genetic diagnostic device can be used to identify individuals, identify criminal investigations, identify parent-child relationships, and ensure the security of each individual.
[0072]
In the genetic diagnostic apparatus according to claim 2, since the closed flow path is a separation closed flow path cartridge, a buffer solution containing a linear polymer and a DNA binding control agent in advance, a separation DNA conjugate, and a delay DNA conjugate. Separation closed channel cartridge filled with gate and DNA sample can be prepared, and it is only necessary to replace and install the separation sealed channel cartridge in the separation section for each measurement, making measurement simple and easy Can be done.
[0073]
Since the genetic diagnosis apparatus according to claim 3 is provided with one or more sealed flow paths, a DNA sample is obtained by changing a delay DNA conjugate, a separation DNA conjugate, and a DNA binding control agent for each sealed flow path. The separation environment of normal DNA and abnormal DNA can be changed for each sealed channel.
[0074]
Since the genetic diagnosis apparatus described in claim 4 includes one or more types of delay DNA conjugates, the migration speed can be changed by changing the ratio of the delay DNA conjugates.
[0075]
In the genetic diagnosis apparatus according to claim 5, since the DNA conjugate for separation and / or the DNA conjugate for delay is vinylized DNA, normal DNA and abnormal DNA of the DNA sample are clearly separated and measured. It becomes possible.
[0076]
In the genetic diagnosis apparatus according to claim 6, the separation unit adjusts the liquid in the interior to 20 ° C. to 60 ° C. to separate normal DNA and abnormal DNA, so that normal DNA and abnormal DNA are separated by temperature adjustment. The conjugate can be bound to or detached from the delay DNA conjugate, the binding force can be adjusted by temperature, and each can be measured by the detection unit after separation.
[0077]
The genetic diagnosis apparatus according to claim 7 is a fused silica capillary tube having an inner diameter of 50 to 100 μm, so that it can transmit ultraviolet light of 90% or more, and detect abnormal DNA by detecting the amount of ultraviolet light passing therethrough. Can be easily detected.
[0078]
The genetic diagnostic device according to claim 8 is a combination of a plate with a grooved groove and a plate that transmits 90% or more of ultraviolet rays, so that it can transmit 90% or more of ultraviolet rays and detect the passing amount of ultraviolet rays. By doing so, abnormal DNA can be easily detected.
[0079]
The invention according to claim 9 is the genetic diagnosis apparatus according to any one of claims 1 to 8, wherein the double-stranded DNA sample is separated to form a single-stranded DNA sample. Since it can be used as it is without pretreatment to make a heavy chain, it is possible to further automate diagnosis.
[0080]
In the genetic diagnosis method described in claim 10, a predetermined constant voltage is applied between the second electrode and the first electrode, and the DNA sample can be electrophoresed. Since the gate is bound to the polymer compound, the migration speed is only a few percent compared to the DNA sample (however, it depends on the type and length of the polymer compound), and is relatively in a pseudo-fixed state. can do. Thus, the DNA sample is electrophoretically passed through the retarding DNA conjugate and then the separating DNA conjugate portion. At that time, first, by using the difference in hydrogen bond strength with the DNA conjugate for delay, the migration speed of normal DNA and abnormal DNA group is reduced with respect to noise DNA, and further, the migration of normal DNA is performed with the DNA conjugate for separation. The speed can be reduced relative to the migration speed of abnormal DNA.
[0081]
Although there is affinity DNA as a method for delaying a DNA sample, it is common to fix affinity DNA on the wall surface of a closed channel such as a capillary tube, and the fixing process is difficult. However, according to the present invention, since it is pseudo-fixed, it is not necessary to make it disposable, and it is very easy to adjust the concentration of both conjugates and samples and the mixing ratio of both conjugates and samples. .
[0082]
While normal DNA and abnormal DNA move, they are first subjected to the action of the binding force of the delay DNA conjugate, and noise DNA that does not receive this action is migrated first when a voltage is applied and detected by the detector. The However, the binding force with the DNA conjugate for separation as well as the DNA conjugate for separation acts on the abnormal DNA (however, it is weaker by one base compared with normal DNA), and the action with the conjugate cannot be easily shaken off. Electrophoresis is performed later than the noise DNA, and is detected by the detection unit next to the noise DNA. The maximum binding force acts on normal DNA, and it migrates later than abnormal DNA as well as noise DNA, and is finally detected by the detection unit. Thereby, a difference can be caused in the detection time of the three DNAs. Since electrophoresis and DNA hydrogen bonding are used, DNA can be separated in a short time of several minutes to several tens of minutes, and it is only necessary to apply a predetermined voltage, so it can be adjusted very easily to an optimum voltage with high resolution. It is possible to accurately detect the presence or absence of DNA abnormality. According to this genetic diagnosis method, it is possible to predict the risk of onset of a disease caused by a gene mutation, prevent it, and detect it at an extremely early stage. In addition, by investigating the diversity of genes possessed by each individual, it is possible to presume in advance whether there are side effects and effects of the drug, and to provide the drug most suitable for each individual. Furthermore, it is possible to quickly determine a mutation of a gene collected from a tissue that has become cancerous. Individuals can be identified, and criminal investigations, identification of parent-child relationships, and the security of each individual can be given definitive reliability.
[0083]
[Sequence Listing]

[Brief description of the drawings]
FIG. 1 is an external view of a genetic diagnosis apparatus according to Embodiment 1 of the present invention.
FIG. 2 is an external view of the open top lid of the genetic diagnosis apparatus according to Embodiment 1 of the present invention.
FIG. 3 is a device configuration diagram of the genetic diagnosis device according to the first embodiment of the present invention.
FIG. 4 is a main part diagram of the control circuit of the genetic diagnosis apparatus according to the first embodiment of the present invention.
FIG. 5 is an introduction state diagram of a separation DNA conjugate, a delaying DNA conjugate, and a DNA sample in a sealed channel of the genetic diagnosis apparatus according to the first embodiment of the present invention.
6A is a conceptual diagram of the relationship between a DNA conjugate for separation and a DNA sample in a sealed channel of the genetic diagnostic apparatus according to Embodiment 1 of the present invention. FIG.
(B) Conceptual diagram of the relationship between the DNA conjugate for delay and the DNA sample in the closed flow path of the genetic diagnostic apparatus in Embodiment 1 of the present invention
FIG. 7 is a relationship diagram between elapsed time and absorbance.
FIG. 8 is an apparatus configuration diagram of a genetic diagnosis apparatus according to Embodiment 2 of the present invention.
[Explanation of symbols]
1 Power switch
2 Operation buttons
3 Display panel
4 Top cover
5 Case
6 Electrophoresis part
7 Support stand
8 Control operation part
9 Power box
9a Power supply
10 High temperature part
11 Heat insulation part
12 Separation part
13 First temperature controller
14 Second temperature controller
15 detector
15a D ₂ lamp
15b photodiode
15c preamplifier
15d A / D converter
16, 17 electrodes
18 Buffer
18a, 18b container
18d linear polymer gel
19 Capillary tube
20 Suction pump
21 DNA conjugate for separation
22 DNA conjugate for delay
23 DNA samples

Claims (10)

A first container containing a buffer solution and immersed in the first electrode;
A second container containing a buffer solution and immersed in the second electrode;
A sealed flow path in which the first container and the second container are filled and filled with a buffer containing a linear polymer and a DNA binding control agent;
A power supply for applying a positive potential to the second electrode and applying a negative potential to the first electrode;
A control unit that controls the power supply unit to apply a predetermined constant voltage between the second electrode and the first electrode;
Provided in the closed flow path, provided with a detection unit for detecting the amount of DNA passing through the inside,
In the closed channel, in the buffer solution,
A DNA conjugate for separation in which a first base sequence capable of hydrogen bonding to a DNA sample is bonded to a polymer compound, and the DNA sample is separated into normal DNA and abnormal DNA from the difference in binding strength;
A delay DNA conjugate in which a second base sequence and a polymer compound are bonded, and the second base sequence has an equivalent binding force to normal DNA and abnormal DNA to distinguish only noise DNA;
In addition, a DNA sample is filled,
A gene diagnostic apparatus, wherein the constant voltage is applied to cause electrophoresis of DNA in the sealed channel, and the detection unit measures the passing amount of normal DNA, abnormal DNA, and noise DNA, respectively. The sealed channel is filled with a buffer solution containing a linear polymer and a DNA binding control agent, and the separation DNA conjugate, the delay DNA conjugate, and the DNA sample are separated in the buffer solution. 2. A sealed flow channel cartridge for separation, which is filled in this order with a linear polymer interposed therebetween, wherein a separation unit is provided to replaceably attach the closed flow channel cartridge for separation. Genetic diagnostic equipment. The genetic diagnosis apparatus according to claim 1, wherein one or more of the sealed flow paths are provided. The genetic diagnosis apparatus according to any one of claims 1 to 3, wherein one or more types of the delay DNA conjugates are contained. The genetic diagnosis apparatus according to any one of claims 1 to 4, wherein the DNA conjugate for separation and / or the DNA conjugate for delay is vinylated DNA. The genetic diagnostic apparatus according to any one of claims 1 to 5, wherein a normal DNA and an abnormal DNA are separated by adjusting a liquid in the sealed channel to 20 to 60 ° C. The genetic diagnosis apparatus according to any one of claims 1 to 6 , wherein the sealed channel is a fused silica capillary tube having an inner diameter of 50 to 100 µm. The genetic diagnosis apparatus according to any one of claims 1 to 6, wherein the sealed flow path is a combination of a plate having a groove and a plate that transmits 90% or more of ultraviolet rays. The genetic diagnosis apparatus according to any one of claims 1 to 8 , further comprising a high-temperature portion that heats the closed channel and separates a double-helix DNA sample to form a single-stranded DNA sample. A buffer solution is stored in the first container and the first electrode is immersed, and a buffer solution is also stored in the second container and the second electrode is immersed, and a linear polymer and DNA are interposed between the first container and the second container. Filled with a buffer containing a binding control agent and communicated in a sealed channel, and then the first base sequence capable of hydrogen bonding to the DNA sample and the polymer compound are contained in the buffer in the sealed channel. The DNA sample is bound and filled with a separation DNA conjugate that separates the DNA sample into normal DNA and abnormal DNA from the difference in binding strength, and then the second base sequence and the polymer compound are combined to form normal DNA and abnormal A DNA conjugate for delaying that distinguishes only noise DNA from DNA having the same binding force with respect to the second base sequence is filled, a DNA sample is added, and then a positive potential is applied to the second electrode. And applying the first electrode A negative potential is applied, by applying a predetermined constant voltage between the second electrode and the first electrode, the DNA samples of the closed flow path are electrophoresed to separate normal DNA and abnormal DNA and noise DNA, A genetic diagnosis method comprising: quantifying normal DNA, quantifying abnormal DNA, or a ratio of normal DNA to abnormal DNA, or detecting abnormal DNA.

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