JP2008134259A - Nucleic acid fixing magnetic particle - Google Patents

Nucleic acid fixing magnetic particle Download PDF

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JP2008134259A
JP2008134259A JP2008024128A JP2008024128A JP2008134259A JP 2008134259 A JP2008134259 A JP 2008134259A JP 2008024128 A JP2008024128 A JP 2008024128A JP 2008024128 A JP2008024128 A JP 2008024128A JP 2008134259 A JP2008134259 A JP 2008134259A
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magnetic particles
nucleic acid
magnetic particle
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acid
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JP4545200B2 (en
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Atsushi Izumi
篤志 泉
Junichi Kosuge
順一 小菅
Masayuki Nozawa
正之 野沢
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Sekisui Medical Co Ltd
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Abstract

<P>PROBLEM TO BE SOLVED: To provide a nucleic acid fixing magnetic particle which keeps the quantity of a fixing nucleic acid per unit of the quantity of magnetic particles increased by introducing a plurality of functional groups on the surface of the magnetic particle, has an excellent dispersion state within an aqueous solution due to a hydrophilicity of the introduced functional groups, and detects a nucleic acid at the high operability and the high sensitivity. <P>SOLUTION: The nucleic acid fixing magnetic particle has a polyacidic amino acid or a polybasic amino acid bonded to the surface through an amide bond. <P>COPYRIGHT: (C)2008,JPO&INPIT

Description

本発明は、表面の官能基量を増加させることにより多量の核酸を固定化することができる、核酸の分離精製や検出に利用される核酸固定用磁性粒子に関する。 The present invention relates to a magnetic particle for immobilizing nucleic acid, which can be used for separation and purification of nucleic acid and detection, which can immobilize a large amount of nucleic acid by increasing the amount of functional groups on the surface .

核酸、蛋白質などの生体内物質を特異的に検出又は精製するには、目的とする生体内物質を特異的に標識又は分離する手段が必要であるが、そのひとつとして固相に目的生体内物質と特異的に結合する性質の物質を固定化し、溶液中の目的物質を特異的に捕獲する方法が広く用いられている(非特許文献1)。特に、核酸の検出又は精製の場合は相補的な核酸が特異的に結合(ハイブリダイゼーション)する性質を利用することによって目的とする核酸を特異的に捕獲することができ、この相補的な核酸を固定化するための固相として、液相中で細かく分散させることにより液相-固相間の高い反応性が得られ、磁石に吸着させることにより簡便に液相と分離できる磁性粒子が用いられるようになっている。 In order to specifically detect or purify in vivo substances such as nucleic acids and proteins, a means for specifically labeling or separating the target in vivo substances is required. A method of immobilizing a substance that specifically binds to the target substance and specifically capturing the target substance in the solution is widely used ( Non-patent Document 1 ). In particular, in the case of detection or purification of a nucleic acid, the target nucleic acid can be specifically captured by utilizing the property that the complementary nucleic acid specifically binds (hybridize). As the solid phase for immobilization, magnetic particles that can be separated from the liquid phase easily by adsorbing to a magnet can be obtained by high dispersion between the liquid phase and solid phase by finely dispersing in the liquid phase. It is like that.

それには、まず目的とする核酸をハイブリダイゼーションによって捕獲するための相補的な核酸を磁性粒子へ固定化する必要がある。核酸を固定化する方法としては、粒子の表面へ物理吸着させる方法と、粒子表面のアミノ基、カルボキシル基などの官能基へ共有結合させる方法が知られている(非特許文献2)。また、ビオチンアビジン系を用いた固定化法も利用されている(非特許文献3)。 For this purpose, it is first necessary to immobilize complementary nucleic acids on the magnetic particles for capturing the target nucleic acid by hybridization. Known methods for immobilizing nucleic acids include a method of physical adsorption to the surface of particles and a method of covalent bonding to functional groups such as amino groups and carboxyl groups on the particle surface ( Non-patent Document 2 ). An immobilization method using a biotin-avidin system is also used ( Non-patent Document 3 ).

物理吸着法は簡便な手法であるが、結合力が弱く、ある種の界面活性剤などを用いた強い条件で洗浄すると核酸が剥離する可能性がある。また、共有結合法は、固定化すべき核酸に官能基を導入する必要があり物理吸着法に比べて操作は煩雑であるが、粒子と核酸とを強く結合させることが可能である(非特許文献2)。共有結合法における粒子表面の官能基としては、カルボキシル基、アミノ基、水酸基などが知られている(非特許文献2)。粒子表面のカルボキシル基は、1-(3-ジエチルアミノプロピル)-3-エチルカルボジイミド塩酸塩(EDC)などの活性化試験薬で活性化し、核酸にあらかじめ導入したアミノアルキル基と結合させることができる。粒子表面のアミノ基は、2価反応性の架橋試薬を用いてカルボキシル基に変換し、核酸にあらかじめ導入したアミノアルキル基と結合させる(非特許文献4)か、又は末端に付加したリン酸と結合させることができる(非特許文献2)。また、粒子表面の水酸基は、トシル基で活性化して核酸に付加したアミノアルキル基と結合させることができる(非特許文献5)。 Although the physical adsorption method is a simple method, the binding force is weak, and the nucleic acid may be detached when washed under strong conditions using a certain kind of surfactant. In addition, the covalent bond method requires introduction of a functional group into the nucleic acid to be immobilized and is more complicated than the physical adsorption method, but can strongly bond the particle and the nucleic acid ( non-patent document). 2 ). As functional groups on the particle surface in the covalent bonding method, a carboxyl group, an amino group, a hydroxyl group, and the like are known ( Non-patent Document 2 ). The carboxyl group on the particle surface can be activated with an activation test agent such as 1- (3-diethylaminopropyl) -3-ethylcarbodiimide hydrochloride (EDC) and bound to an aminoalkyl group previously introduced into the nucleic acid. The amino group on the particle surface is converted to a carboxyl group using a divalent reactive crosslinking reagent and bonded to an aminoalkyl group previously introduced into the nucleic acid ( Non-patent Document 4 ), or phosphoric acid added to the terminal. They can be combined ( Non-Patent Document 2 ). Further, the hydroxyl group on the particle surface can be bound to an aminoalkyl group activated by a tosyl group and added to a nucleic acid ( Non-patent Document 5 ).

これらのうち、粒子表面にカルボキシル基を有する磁性粒子を利用する方法は、反応性も高く、効率よく核酸を導入することが可能であるが、核酸に導入したアミノアルキル基との反応の選択性に問題があり、実際にハイブリダイゼーションに有効な状態で結合している核酸は少ない(非特許文献2)。一方、粒子表面にアミノ基を有する磁性粒子を利用して2価反応性架橋試薬を用いる方法は、副反応が少なく核酸に付加したアミノアルキル基と特異的に反応するため核酸を有効に結合させることが可能である。しかし、一般的にアミノ基の付加した磁性粒子を利用した場合、カルボキシル基の付加したものに比べて導入できる核酸の量が少ないという問題がある。特に、磁性粒子法と化学発光検出法(非特許文献6)を組合せて用いる場合は、磁性粒子による溶液の濁りが発光検出を阻害するため、使用粒子量をできうる限り少なくする必要があり、十分量の固定化核酸を利用するためには単位粒子量当たりの核酸の固定量を上げる必要がある。 Among these, the method using magnetic particles having a carboxyl group on the particle surface has high reactivity and can efficiently introduce a nucleic acid, but the selectivity of the reaction with an aminoalkyl group introduced into the nucleic acid. There are few nucleic acids that are actually bound in a state effective for hybridization ( Non-patent Document 2 ). On the other hand, the method using a divalent reactive cross-linking reagent using magnetic particles having amino groups on the particle surface effectively binds nucleic acids because there are few side reactions and specifically reacts with aminoalkyl groups added to the nucleic acids. It is possible. However, in general, when magnetic particles to which amino groups are added are used, there is a problem that the amount of nucleic acid that can be introduced is smaller than those to which carboxyl groups are added. In particular, when the magnetic particle method and the chemiluminescence detection method ( Non-Patent Document 6 ) are used in combination, the turbidity of the solution due to the magnetic particles hinders luminescence detection, so the amount of particles used needs to be as small as possible. In order to use a sufficient amount of immobilized nucleic acid, it is necessary to increase the amount of nucleic acid immobilized per unit particle amount.

一方、磁性粒子としては、ポリスチレンなどの疎水性の素材をベースとして用いたものが知られているが(非特許文献2)、それらのものは水溶液中で疎水的に凝集を起こしやすく、また容器の壁に吸着し、水溶液中への分散及び磁石への集合が阻害される。また、蛋白質、核酸などを非特異的に吸着しやすいために、生体内物質の検出に使用する場合はバックグラウンドの上昇の原因となることが考えられる。 On the other hand, as magnetic particles, those using a hydrophobic material such as polystyrene as a base are known ( Non-patent Document 2 ), but these particles are easily agglomerated in an aqueous solution. Adhering to the wall of the metal, the dispersion in the aqueous solution and the assembly into the magnet are hindered. In addition, since proteins, nucleic acids and the like are easily adsorbed non-specifically, it may cause an increase in background when used for detection of in-vivo substances.

千葉仁志,ニッポン臨床53巻9号(9, 1995)Hitoshi Chiba, Nippon Clinical 53, 9 (9, 1995) Vera Land, Ruth Schmid, David Rickwood, Erik Hornes(1988). Nucleic Acids Res. 16(22), 10861Vera Land, Ruth Schmid, David Rickwood, Erik Hornes (1988) .Nucleic Acids Res. 16 (22), 10861 Shao-Ochie Huang, Harold Swerclow, and Karin D. Caldwell(1994). Analytical Biochemistry 222, 441-119Shao-Ochie Huang, Harold Swerclow, and Karin D. Caldwell (1994) .Analytical Biochemistry 222, 441-119 Running, J. A., Urdea, N. S.,(1990) Bio Techniques 8,(3), 276Running, J. A., Urdea, N. S., (1990) Bio Techniques 8, (3), 276 Yu-An Chang, Adrian Gee, Alan Smith, William Lake(1992) Bioconjugate Chem. 3, 200-202Yu-An Chang, Adrian Gee, Alan Smith, William Lake (1992) Bioconjugate Chem. 3, 200-202 Debbie J. Berry, Penelope M. S. Clark, and Christopher P. Price(1998) Clin. Chem. 34(10), 2087-2090Debbie J. Berry, Penelope M. S. Clark, and Christopher P. Price (1998) Clin. Chem. 34 (10), 2087-2090

そこで、本発明は、磁性粒子表面に多くの官能基を導入することによって、単位磁性粒子量当たりの固定化核酸量が向上すると共に、導入した官能基の親水性により水溶液中での分散状態にも優れ高感度で操作性の良い核酸検出が可能な核酸固定用磁性粒子を提供することを目的とする。 Accordingly, the present invention can be prepared by introducing many functional groups on the magnetic particle surface, with the immobilized nucleic acid per unit magnetic particle amount is increased, introduced functional groups in I Rimizu solution a hydrophilic An object of the present invention is to provide a magnetic particle for immobilizing nucleic acid which is excellent in dispersion state, capable of detecting nucleic acid with high sensitivity and good operability.

かかる実情において本発明者らは、多官能基を持つポリマー、特にポリアミノ酸中に核酸を結合させるために有用なアミノ基又はカルボキシル基が多量に存在し、かつ親水性も高いことに注目し、これらのポリマーを磁性粒子表面に結合又は被覆することによって核酸固定化量を増やすことができると共に、ポリマー分子の親水性によって磁性粒子の水溶液中での分散状態が改善されることを見出した。また、特に表面にカルボキシル基を有する磁性粒子にポリ塩基性アミノ酸を結合させれば、導入核酸量が少ないというアミノ基を有する磁性粒子の欠点及び直接核酸を固定化すると副反応を起こす可能性が高いというカルボキシル基を有する磁性粒子の欠点の双方を補い、核酸を効果的かつ効率的に導入することが可能となることを見出し、本発明を完成した。   In such a situation, the present inventors pay attention to the presence of a large amount of amino groups or carboxyl groups useful for binding a nucleic acid in a polymer having a polyfunctional group, particularly a polyamino acid, and high hydrophilicity. It has been found that the amount of nucleic acid immobilized can be increased by binding or coating these polymers on the surface of the magnetic particles, and the dispersion state of the magnetic particles in the aqueous solution is improved by the hydrophilicity of the polymer molecules. In particular, if a polybasic amino acid is bound to magnetic particles having a carboxyl group on the surface, the amount of introduced nucleic acid is small, and the disadvantage of magnetic particles having amino groups is that there is a possibility of causing side reactions when directly immobilizing nucleic acids. The present invention was completed by discovering that it is possible to effectively and efficiently introduce nucleic acids by making up for both of the disadvantages of magnetic particles having a high carboxyl group.

すなわち本発明は、表面にアミド結合を介してポリ酸性アミノ酸又はポリ塩基性アミノ酸が結合してなる核酸固定用磁性粒子を提供するものである。 That is, the present invention provides magnetic particles for immobilizing nucleic acids, which are formed by binding polyacidic amino acids or polybasic amino acids to the surface via amide bonds .

本発明の核酸固定用磁性粒子は、以下のような効果を有する。 The magnetic particle for immobilizing nucleic acid of the present invention has the following effects.

(1) 本発明によれば、従来の方法に比べて磁性粒子に格段に多量の核酸を効果的に固定化することが可能である。従って、目的とする核酸を効率的に捕獲することが可能であり、核酸検出の測定感度が向上する。 (1) According to the present invention, it is possible to immobilize a much larger amount of nucleic acid on magnetic particles more effectively than conventional methods. Therefore, it is possible to efficiently capture the target nucleic acid, and the measurement sensitivity for nucleic acid detection is improved.

(2) 本発明によれば、単位磁性粒子量当たりの有効な核酸の固定化量を格段に増やすことができるため、同一の測定当たりに使用する磁性粒子の量を減らすことができる。従って、磁性粒子による溶液の濁度を減らすことができるため、特に検出システムとして化学発光を採用している場合、検出光量が増加し、感度が向上する。 (2) According to the present invention, the effective immobilization amount of nucleic acid per unit magnetic particle amount can be remarkably increased, so that the amount of magnetic particles used for the same measurement can be reduced. Therefore, since the turbidity of the solution due to the magnetic particles can be reduced, particularly when chemiluminescence is employed as the detection system, the amount of detected light is increased and the sensitivity is improved.

(3) 本発明によれば、疎水性材質で被覆された磁性粒子が水溶性のポリマーで被覆されるため、水溶液中での磁性粒子の分散性が向上する。 (3) According to the present invention, since the magnetic particles coated with a hydrophobic material are coated with a water-soluble polymer, the dispersibility of the magnetic particles in an aqueous solution is improved.

(4) 本発明によれば、疎水性材質で被覆された磁性粒子が水溶性のポリマーで被覆されるため、検出目的とする核酸以外の生体内物質などの磁性粒子への非特異的な吸着が防止され、測定時のノイズレベルが減少する。 (4) According to the present invention, since magnetic particles coated with a hydrophobic material are coated with a water-soluble polymer, non-specific adsorption to magnetic particles such as in vivo substances other than nucleic acids to be detected Is prevented, and the noise level during measurement is reduced.

(5) 本発明によれば、従来の磁性粒子の疎水性固相表面と固定化核酸の間に、ポリマー分子又は複数連結を繰り返したポリマー分子を介しているため、検出対象とする核酸と磁性粒子上の固定化核酸分子との接近が容易になり、ハイブリダイゼーション反応の効率が向上し、検出感度を高くすることが可能となる。 (5) According to the present invention, since a polymer molecule or a polymer molecule in which multiple linkages are repeated is interposed between the hydrophobic solid phase surface of a conventional magnetic particle and the immobilized nucleic acid, the nucleic acid to be detected and the magnetic Access to the immobilized nucleic acid molecule on the particle is facilitated, the efficiency of the hybridization reaction is improved, and the detection sensitivity can be increased.

以下、本発明を詳細に説明する。まず、磁性粒子に多官能基を有するポリマーを結合させる方法について説明する。   Hereinafter, the present invention will be described in detail. First, a method for bonding a polymer having a polyfunctional group to magnetic particles will be described.

本発明に使用される磁性粒子としては、ローヌプーラン社のエスタポール、セラダイン社のCM-MP、パーセプティブ社のバイオマグ、日本ペイント社のフェリスフェアなど、磁性粒子表面にアミノ基又はカルボキシル基を有するものが好ましい。また、ダイナテック社のダイナビーズなど、磁性粒子表面の官能基が水酸基のものも、3-アミノプロピルトリエトキシシラン等の試薬を利用してアミノアルキル基を導入して用いることができる。   Examples of the magnetic particles used in the present invention include those having an amino group or a carboxyl group on the surface of the magnetic particles, such as Rhône-Poulenc Estapol, Ceradyne CM-MP, Perceptive Biomag, Nippon Paint Ferrissphere, etc. Is preferred. Also, Dynabe Corp.'s Dynabeads having a functional group on the surface of magnetic particles having a hydroxyl group can be used by introducing an aminoalkyl group using a reagent such as 3-aminopropyltriethoxysilane.

表面にカルボキシル基を有する磁性粒子と反応させる場合に用いられる、カルボキシル基と反応する官能基を3個以上有する多官能基性ポリマーとしては、ポリ塩基性アミノ酸、例えばポリD-リジン、ポリL-リジン、ポリDL-リジン;ポリD-オルニチン、ポリL-オルニチン、ポリDL-オルニチン;ポリエチレンイミン、ポリ(トリメチレンイミン)等のポリアルキルイミン;又はそれらの塩酸塩、硫酸塩、臭化水素塩、コハク酸塩などが挙げられ、なかでもポリリジン及びポリオルニチン、更にポリD-リジン及びポリD-オルニチン、特にポリD-リジンが好ましい。またこれらのポリマーをN-サクシンイミジル-S-アセチルチオアセテート等の試薬と反応させることにより、アミノ基をチオール基に変換させたものを用いることも可能である。一方、表面にアミノ基を有する磁性粒子と反応させる場合に用いられる、アミノ基と反応する官能基を3個以上有する多官能基性ポリマーとしては、ポリ酸性アミノ酸、例えばポリD-グルタミン酸、ポリL-グルタミン酸、ポリDL-グルタミン酸;ポリD-アスパラギン酸、ポリL-アスパラギン酸、ポリDL-アスパラギン酸;又はそれらのナトリウム塩、カリウム塩等が挙げられ、なかでもポリD-グルタミン酸及びポリD-アスパラギン酸が好ましい。更に、ポリ(リジン-アラニン)、ポリ(グルタミン酸-アラニン)等のリジン、グルタミン酸、アスパラギン酸を含むアミノ酸のポリマー又はその塩でもよい。   Polybasic amino acids such as poly-D-lysine, poly-L-, which are used when reacting with magnetic particles having a carboxyl group on the surface and have three or more functional groups that react with carboxyl groups, are used as polybasic amino acids. Lysine, poly-DL-lysine; poly-D-ornithine, poly-L-ornithine, poly-DL-ornithine; polyalkylimines such as polyethyleneimine, poly (trimethyleneimine); or their hydrochlorides, sulfates, hydrobromides Succinate, and the like. Among them, polylysine and polyornithine, poly D-lysine and poly D-ornithine, particularly poly D-lysine are preferred. It is also possible to use those obtained by reacting these polymers with a reagent such as N-succinimidyl-S-acetylthioacetate to convert an amino group into a thiol group. On the other hand, polyacidic polymers having three or more functional groups that react with amino groups used when reacting with magnetic particles having amino groups on the surface include polyacidic amino acids such as poly-D-glutamic acid, poly-L -Glutamic acid, poly DL-glutamic acid; poly D-aspartic acid, poly L-aspartic acid, poly DL-aspartic acid; or their sodium salts, potassium salts, etc. Acid is preferred. Further, it may be a polymer of amino acids containing lysine such as poly (lysine-alanine) and poly (glutamic acid-alanine), glutamic acid and aspartic acid, or a salt thereof.

表面にカルボキシル基を有する磁性粒子に多官能基性ポリマーを反応させるには、まず磁性粒子のカルボキシル基を活性化する必要がある。磁性粒子のカルボキシル基の活性化は、磁性粒子を分散させた弱酸性又は中性付近の水溶液又は緩衝液中に活性化剤を加え、室温で30分程度振盪した後、磁石で磁性粒子を分離し、水又は緩衝液で洗浄して過剰の試薬を取り除くことにより行われる。活性化剤としては、1,3-ジシクロヘキシルカルボジイミド及び1-(3-ジエチルアミノプロピル)-3-エチルカルボジイミド塩酸塩が好ましいものとして挙げられる。活性化磁性粒子と多官能基性ポリマーとの反応は、活性化磁性粒子に、そのカルボキシル基に対して大過剰の多官能基性ポリマー(ポリ塩基性アミノ酸)を緩衝液に溶解したものを加え、適当な条件で振盪することにより行われる。反応後、磁石で磁性粒子を分離して溶液を取り除き、未反応のポリマーを塩化ナトリウム水溶液及び緩衝液で洗浄して、アミノ基を多数有するポリ塩基性アミノ酸結合磁性粒子を得ることができる。   In order to react a polyfunctional polymer with magnetic particles having a carboxyl group on the surface, it is first necessary to activate the carboxyl groups of the magnetic particles. Activation of the carboxyl group of the magnetic particles is achieved by adding an activator to a weakly acidic or neutral aqueous solution or buffer in which the magnetic particles are dispersed, shaking for 30 minutes at room temperature, and then separating the magnetic particles with a magnet. And washing with water or buffer to remove excess reagent. Preferred activators include 1,3-dicyclohexylcarbodiimide and 1- (3-diethylaminopropyl) -3-ethylcarbodiimide hydrochloride. The reaction between the activated magnetic particles and the polyfunctional polymer is performed by adding a large excess of polyfunctional polymer (polybasic amino acid) in the buffer to the activated magnetic particles. , By shaking under appropriate conditions. After the reaction, the magnetic particles are separated with a magnet to remove the solution, and the unreacted polymer is washed with an aqueous sodium chloride solution and a buffer solution to obtain polybasic amino acid-bonded magnetic particles having many amino groups.

更に、上記の表面にカルボキシル基を有する磁性粒子として、表面にアミノ基を有する磁性粒子の懸濁溶液に、環状酸無水物、好ましくは無水コハク酸を反応させることによりカルボキシル基を導入した磁性粒子を用い、このものに対して上記と同様にポリ塩基性アミノ酸を結合させることも可能である。また以上のようにして得られたアミノ基を多数有するポリ塩基性アミノ酸結合磁性粒子の懸濁溶液に、環状酸無水物、好ましくは無水コハク酸を反応させることにより、カルボキシル基を導入することもできる。このものに対して上記と同様にポリ塩基性アミノ酸を結合させることによって更に官能基数の増幅を図ることが可能である。   Furthermore, as magnetic particles having a carboxyl group on the surface, magnetic particles having a carboxyl group introduced by reacting a suspension of magnetic particles having an amino group on the surface with a cyclic acid anhydride, preferably succinic anhydride. It is also possible to bind a polybasic amino acid to this product in the same manner as described above. Alternatively, a carboxyl group may be introduced by reacting a suspension of polybasic amino acid-bonded magnetic particles having a large number of amino groups obtained as described above with a cyclic acid anhydride, preferably succinic anhydride. it can. It is possible to further amplify the number of functional groups by attaching a polybasic amino acid to this product in the same manner as described above.

また、表面にアミノ基を有する磁性粒子に多官能基性ポリマーを反応させるには、まず多官能基性ポリマー(ポリ酸性アミノ酸)のカルボキシル基を活性化する必要がある。ポリ酸性アミノ酸のカルボキシル基の活性化は、ポリ酸性アミノ酸をDMF、DMSO、アセトニトリル等の無水の有機溶媒に懸濁し、前記と同様の活性化剤を加えて室温で30分程度振盪することにより行われる。これを表面にアミノ基を有する磁性粒子の懸濁溶液に加えて反応させることにより、カルボキシル基を多数有するポリ酸性アミノ酸結合磁性粒子を得ることができる。   In order to react a polyfunctional polymer with magnetic particles having amino groups on the surface, it is first necessary to activate the carboxyl group of the polyfunctional polymer (polyacidic amino acid). Activation of the carboxyl group of the polyacidic amino acid is carried out by suspending the polyacidic amino acid in an anhydrous organic solvent such as DMF, DMSO, acetonitrile, etc., adding the same activator as described above, and shaking at room temperature for about 30 minutes. Is called. By adding this to a suspension of magnetic particles having amino groups on the surface and reacting them, it is possible to obtain polyacidic amino acid-bonded magnetic particles having many carboxyl groups.

また、上記のようにして得られたカルボキシル基を多数有するポリ酸性アミノ酸結合磁性粒子に、更にポリ塩基性アミノ酸を結合することによって、官能基の数をより増幅することも可能である。この場合の磁性粒子の活性化及びポリ塩基性アミノ酸との反応は前記と同様にして行うことができる。   It is also possible to further amplify the number of functional groups by further binding a polybasic amino acid to the polyacidic amino acid-bonded magnetic particles having a large number of carboxyl groups obtained as described above. In this case, the activation of the magnetic particles and the reaction with the polybasic amino acid can be performed in the same manner as described above.

また、ポリ塩基性アミノ酸を結合させた磁性粒子に、更にポリ酸性アミノ酸を活性化し、結合することによって、官能基の数を増幅することも可能である。   It is also possible to amplify the number of functional groups by further activating and binding polyacidic amino acids to magnetic particles to which polybasic amino acids are bound.

なお、最終的に磁性粒子表面の官能基をカルボキシル基とし、これを核酸の検出や精製に使用する場合、この磁性粒子は、それに結合している多数のカルボキシル基を活性化することによって、アミノアルキル基を有する核酸、又はその他の生理活性物質を結合させることを目的としているが、このとき粒子表面にアミノ基が残存していると、これが活性化されたカルボキシル基と反応して、目的物との反応を阻害する。そこで、この磁性粒子の懸濁溶液に無水酢酸、無水コハク酸、スルホサクシンイミジルアセテート等のキャッピング剤を加え、残存アミノ基を塞ぐことにより、不活性化することが好ましく、これにより、活性化したカルボキシル基に目的とする核酸等の生理活性物質を効率よく結合させることができる。   When the functional group on the surface of the magnetic particle is finally converted into a carboxyl group, and this is used for detection or purification of nucleic acid, the magnetic particle activates a number of carboxyl groups bonded to the amino group. The purpose is to bind a nucleic acid having an alkyl group or other physiologically active substance. At this time, if an amino group remains on the particle surface, it reacts with the activated carboxyl group, and the target product. Inhibits the reaction. Therefore, it is preferable to inactivate by adding a capping agent such as acetic anhydride, succinic anhydride, sulfosuccinimidyl acetate, etc. to the suspension solution of the magnetic particles and blocking the remaining amino groups. Thus, a physiologically active substance such as a target nucleic acid can be efficiently bound to the carboxyl group.

以上の操作を組合せて繰り返し行えば、磁性粒子表面に、親水性の多官能基を持つポリマーの層を積み重ねることができる。   By repeating the above operations in combination, a polymer layer having a hydrophilic polyfunctional group can be stacked on the surface of the magnetic particles.

以上説明した方法により得られる多官能基性磁性粒子のうち、本発明の核酸検出法に使用する上で最も好ましいものは、最終的に磁性粒子表面の官能基をアミノ基としたものであり、このような磁性粒子を用いることにより、導入核酸量が少ないというアミノ基を有する磁性粒子の欠点及び直接核酸を固定化すると副反応を起こす可能性が高いというカルボキシル基を有する磁性粒子の欠点の双方を補い、核酸を効果的かつ効率的に導入することが可能である。   Among the polyfunctional magnetic particles obtained by the method described above, the most preferable ones for use in the nucleic acid detection method of the present invention are those in which the functional group on the surface of the magnetic particles is finally an amino group, By using such magnetic particles, both of the disadvantages of magnetic particles having an amino group that the amount of introduced nucleic acid is small and the disadvantages of magnetic particles having a carboxyl group that are likely to cause a side reaction when nucleic acid is directly immobilized are used. It is possible to effectively and efficiently introduce nucleic acids.

本発明の核酸検出法に用いられる磁性粒子は、上記のようにして得られた多官能基性磁性粒子に、核酸を結合させることによって得ることができる。核酸には、結合に利用するための官能基をあらかじめ導入しておいてもよい(Vera Land, Ruth Schmid, David Rickwood, Erik Hornes(1988). Nucleic Acids Res. 16(22),10861)。導入する官能基は、アミノアルキル基、カルボキシル基、リン酸基など、磁性粒子に導入した官能基と直接反応するもの、又は2価反応性の架橋試薬を利用して間接的に結合させることができるものでもよく、合成的に、又は酵素反応を利用して導入することができる。多官能基性磁性粒子と核酸との結合法としては、ペプチド合成法に用いられるカルボジイミド法、活性エステル法、混酸無水物法等を用いることができる。また間接法の例を挙げれば、合成アミノアルキル化DNAプローブに2価反応性の活性エステルであるジサクシンイミジルスベレートを反応させて活性化DNAプローブとし、これを多数のアミノ基を有するポリマーを結合させた磁性粒子と反応させることにより核酸固定化磁性粒子を得ることができる。更に、その他の結合法としてグルタルアルデヒド法、2,4,6-トリクロロ-s-トリアジン法等を用いることもできる。   The magnetic particles used in the nucleic acid detection method of the present invention can be obtained by binding nucleic acids to the polyfunctional magnetic particles obtained as described above. A functional group for use in binding may be introduced in advance into the nucleic acid (Vera Land, Ruth Schmid, David Rickwood, Erik Hornes (1988). Nucleic Acids Res. 16 (22), 10861). The functional group to be introduced may react directly with a functional group introduced into the magnetic particle such as an aminoalkyl group, a carboxyl group, or a phosphate group, or may be indirectly bonded using a divalent reactive crosslinking reagent. It can also be introduced synthetically or by using an enzymatic reaction. As a method for binding the polyfunctional magnetic particles to the nucleic acid, a carbodiimide method, an active ester method, a mixed acid anhydride method, or the like used for peptide synthesis can be used. As an example of the indirect method, a synthetic aminoalkylated DNA probe is reacted with a divalent reactive active ester, disuccinimidyl suberate to form an activated DNA probe, which is a polymer having many amino groups. Nucleic acid-immobilized magnetic particles can be obtained by reacting with the magnetic particles to which is bound. Further, as other bonding methods, a glutaraldehyde method, a 2,4,6-trichloro-s-triazine method, or the like can be used.

本発明の核酸検出法においては、標識として、放射性物質、蛍光もしくは発光物質、又は酵素を用いることができる。すなわち、ハイブリダイゼーション法を用い、又は組合せて、磁性粒子に固定化した核酸プローブに目的とする核酸を固定化し、更に標識のついた核酸をハイブリダイゼーションさせ、磁石で磁性粒子を分離することによって、磁性粒子上の標識を特異的に検出することができる。   In the nucleic acid detection method of the present invention, a radioactive substance, a fluorescent or luminescent substance, or an enzyme can be used as a label. That is, by using or combining the hybridization method, the target nucleic acid is immobilized on the nucleic acid probe immobilized on the magnetic particles, the labeled nucleic acid is further hybridized, and the magnetic particles are separated with a magnet, The label on the magnetic particle can be specifically detected.

本発明の核酸検出法に用いるハイブリダイゼーション法は、溶液温度を30℃から99℃、好ましくは45℃から70℃まで上昇させた後冷却し、好ましくは25℃付近まで下げることによって、行うことができる。   The hybridization method used in the nucleic acid detection method of the present invention can be performed by raising the solution temperature from 30 ° C. to 99 ° C., preferably from 45 ° C. to 70 ° C., then cooling, and preferably lowering to around 25 ° C. it can.

また、標識に使う酵素としては、アルカリフォスファターゼ、パーオキシダーゼ、β-ガラクトシダーゼ、グルコースオキシダーゼなどが挙げられる。   Examples of the enzyme used for labeling include alkaline phosphatase, peroxidase, β-galactosidase, and glucose oxidase.

また、基質としては、それぞれの酵素に適合した基質を採用することができる。例えば、アルカリフォスファターゼにはp-ニトロフェニルフォスフェート、3-(2′-ピロ-トリサイクロ[3.3.1.1]デカン)-4-メトキシ-4-(3″-フォスフォリルオキシ)フェニル-1,2-ジオキセタン二ナトリウム塩など、パーオキシダーゼには2,2′-アジノビス(3-エチルベンゾチアゾリン-6-スルホン酸(ABTS)、ルミノール-過酸化水素など、β-ガラクトシダーゼにはp-ニトロフェニル-β-o-ガラクトース、3-(2′-スピロアダマンタン)-4-(3-β-D-ガラクトピラノシル)フェニル-1,2-ジオキセタンなどを用いることができる。   Moreover, as a substrate, a substrate suitable for each enzyme can be employed. For example, alkaline phosphatase includes p-nitrophenyl phosphate, 3- (2′-pyro-tricyclo [3.3.1.1] decane) -4-methoxy-4- (3 ″ -phosphoryloxy) phenyl-1, 2-dioxetane disodium salt, 2,2'-azinobis (3-ethylbenzothiazoline-6-sulfonic acid (ABTS) for peroxidase, luminol-hydrogen peroxide, etc., p-nitrophenyl- for β-galactosidase β-o-galactose, 3- (2′-spiroadamantane) -4- (3-β-D-galactopyranosyl) phenyl-1,2-dioxetane, and the like can be used.

検出は、酵素反応が阻害されない温度で行い、生じる発色又は発光量を測定する。   The detection is performed at a temperature at which the enzyme reaction is not inhibited, and the generated color or luminescence amount is measured.

以下、実施例を挙げて本発明をより具体的に説明するが、本発明はこれら実施例に限定されるものではない。   EXAMPLES Hereinafter, although an Example is given and this invention is demonstrated more concretely, this invention is not limited to these Examples.

実施例1 バイオマグアミンへポリグルタミン酸を結合した磁性粒子BM-Eの作製:
ポリ-D-グルタミン酸のナトリウム塩2mgを無水DMF 0.1mlに懸濁し、1-(3-ジエチルアミノプロピル)-3-エチルカルボジイミド塩酸塩(EDC)1.2mgを加え、30分室温で撹拌した。これを、反応容器に磁性粒子バイオマグアミン(官能基はアミノ基,パーセプティブ社製)2mgを100mMリン酸バッファー(pH7.8)1mlに懸濁したものに加えて室温で2時間撹拌した。磁性粒子を1M塩化ナトリウム水と水で洗浄し、100mMリン酸バッファー(pH7.8)1mlに懸濁した後、無水コハク酸2mgを無水DMF 0.1mlに溶解したものを加えて2時間室温で撹拌し、水で磁性粒子を洗浄した。(0.1%SDS,0.15M塩化ナトリウム,15mMクエン酸バッファー)0.2mlに懸濁し、4℃で保存した。
Example 1 Production of magnetic particles BM-E in which polyglutamic acid is bound to biomagamine:
2 mg of sodium salt of poly-D-glutamic acid was suspended in 0.1 ml of anhydrous DMF, 1.2 mg of 1- (3-diethylaminopropyl) -3-ethylcarbodiimide hydrochloride (EDC) was added, and the mixture was stirred at room temperature for 30 minutes. This was added to a reaction vessel in which 2 mg of magnetic particle biomagamine (functional group is amino group, manufactured by Perceptive) was suspended in 1 ml of 100 mM phosphate buffer (pH 7.8) and stirred at room temperature for 2 hours. The magnetic particles were washed with 1M sodium chloride water and water, suspended in 1 ml of 100 mM phosphate buffer (pH 7.8), 2 mg of succinic anhydride dissolved in 0.1 ml of anhydrous DMF was added, and the mixture was stirred for 2 hours at room temperature. The magnetic particles were washed with water. It was suspended in 0.2 ml (0.1% SDS, 0.15 M sodium chloride, 15 mM citrate buffer) and stored at 4 ° C.

実施例2 磁性粒子BM-Eへポリリジンを結合した磁性粒子BM-EKの作製:
反応容器に実施例1で作製したポリグルタミン酸結合磁性粒子BM-Eの20mgを100mM 2-(N-モルホリノ)エタンスルホン酸バッファー(pH6.1,MESバッファー)10mlに懸濁し、磁石で分離した後、液相を除去する操作を繰り返すことによって洗浄した。この操作を2回繰り返した後、100mM N-ヒドロキシサクシンイミドバッファー(pH6.1,HOSuバッファー)10mMに懸濁して、EDC 400mgを加え、室温で30分振盪して、磁性粒子を水で洗浄した。これにポリ-D-リジン臭化水素塩10mgを100mMトリエチルアミン酢酸バッファー(pH7.8)に溶解したものを加え、室温で2時間振盪した。その後、磁性粒子を1M塩化ナトリウム水及び水で洗浄し、(0.1%SDS,0.15M塩化ナトリウム,15mMクエン酸バッファー)1mlに懸濁し、4℃で保存した。
Example 2 Preparation of magnetic particle BM-EK in which polylysine is bonded to magnetic particle BM-E:
After 20 mg of the polyglutamic acid-bonded magnetic particles BM-E prepared in Example 1 were suspended in 10 ml of 100 mM 2- (N-morpholino) ethanesulfonic acid buffer (pH 6.1, MES buffer) in a reaction vessel and separated with a magnet The washing was performed by repeating the operation of removing the liquid phase. After repeating this operation twice, the suspension was suspended in 10 mM of 100 mM N-hydroxysuccinimide buffer (pH 6.1, HOSu buffer), added with 400 mg of EDC, shaken at room temperature for 30 minutes, and the magnetic particles were washed with water. . To this was added 10 mg of poly-D-lysine hydrobromide dissolved in 100 mM triethylamine acetate buffer (pH 7.8), and the mixture was shaken at room temperature for 2 hours. Thereafter, the magnetic particles were washed with 1 M sodium chloride water and water, suspended in 1 ml (0.1% SDS, 0.15 M sodium chloride, 15 mM citrate buffer), and stored at 4 ° C.

試験例1 磁性粒子バイオマグアミンと磁性粒子BM-EK(実施例2)に結合しているアミノ基の量のニンヒドリン発色による比較:
磁性粒子バイオマグアミンと実施例2で作製したポリグルタミン酸−ポリリジン結合磁性粒子BM-EKをそれぞれ水及びメタノールで洗浄し、減圧乾燥した。0.0002Mシアン化カリウムのピリジン溶液200μl、76%フェノールのエタノール溶液100μl及び0.28Mニンヒドリンエタノール溶液100μlを加えて100℃で5分間放置し、60%エタノール3mlを加えて反応を止めた。磁性粒子を分離し、溶液の570nmの吸収を測定したところ、それぞれ0.188,0.363であった。別にコントロールとして磁性粒子を入れずに同様の操作をしたものについて570nmの吸光度を測定したところ、0.016であった。残った磁性粒子をメタノールで洗浄し、乾燥させて重量を測定したところ、それぞれ9.1mg,8.7mgであった。各磁性粒子の1mg当たりのニンヒドリン発色を計算した結果を表1に示す。
Test Example 1 Comparison of the amount of amino groups bound to magnetic particle biomagamine and magnetic particle BM-EK (Example 2) by ninhydrin coloring:
The magnetic particle biomagamine and the polyglutamic acid-polylysine-bonded magnetic particle BM-EK prepared in Example 2 were washed with water and methanol, respectively, and dried under reduced pressure. 200 μl of 0.0002 M potassium cyanide pyridine solution, 100 μl of 76% phenol ethanol solution and 100 μl of 0.28 M ninhydrin ethanol solution were added and left at 100 ° C. for 5 minutes, and the reaction was stopped by adding 3 ml of 60% ethanol. The magnetic particles were separated, and the absorption at 570 nm of the solution was measured and found to be 0.188 and 0.363, respectively. Separately, as a control, the absorbance at 570 nm was measured for the same operation without adding magnetic particles, and found to be 0.016. The remaining magnetic particles were washed with methanol, dried, and weighed to find 9.1 mg and 8.7 mg, respectively. Table 1 shows the results of calculating the ninhydrin color per mg of each magnetic particle.

Figure 2008134259
Figure 2008134259

表1から、ポリリジンを結合させることによってアミノ酸の量が増加していることが確認された。   From Table 1, it was confirmed that the amount of amino acids was increased by binding polylysine.

実施例3 磁性粒子BM-EKへDNAプローブを固定化した磁性粒子BM-EK-DNAの作製:
5′末端にアミノアルキル基を結合した20鎖長のDNAプローブA、0.625ODを100mMトリエチルアミン酢酸バッファー(pH7.8)50μlに溶解し、DMF 50μlを加えてジサクシンイミジルスベレート1mgをDMF 50μlに溶解したものを加え、10分間室温で撹拌した。これに水0.4mlを加えて、酢酸エチル0.4mlで洗浄し、有機溶媒層を取り除く操作を2回繰り返した。これをイソブタノール0.4mlで2回洗浄し、水0.2mlを加えて、100mMリン酸バッファー(pH7.8)3mlに懸濁した実施例2で作製した磁性粒子BM-EK 10mgに加えて4時間室温で撹拌した。磁性粒子を1N塩化ナトリウム水及び水で洗浄して、100mMリン酸バッファー(pH7.8)3mlに懸濁し、スルホサクシンイミジルアセテート8mgを加えて室温で4時間反応させた。1N塩化ナトリウム水及び水で洗浄して(0.1%SDS,0.15M塩化ナトリウム,15mMクエン酸バッファー)0.2mlに懸濁し、4℃で保存した。
Example 3 Production of magnetic particle BM-EK-DNA in which a DNA probe is immobilized on magnetic particle BM-EK:
Dissolve 20-chain DNA probe A, 0.625OD with aminoalkyl group at the 5 'end in 50 μl of 100 mM triethylamine acetate buffer (pH 7.8), add 50 μl of DMF, and add 1 μg of disuccinimidyl suberate to 50 μl of DMF. What was dissolved in was added and stirred at room temperature for 10 minutes. The operation of adding 0.4 ml of water, washing with 0.4 ml of ethyl acetate, and removing the organic solvent layer was repeated twice. This was washed twice with 0.4 ml of isobutanol, added with 0.2 ml of water, suspended in 3 ml of 100 mM phosphate buffer (pH 7.8) and added to 10 mg of the magnetic particles BM-EK prepared in Example 2 for 4 hours. Stir at room temperature. The magnetic particles were washed with 1N sodium chloride water and water, suspended in 3 ml of 100 mM phosphate buffer (pH 7.8), added with 8 mg of sulfosuccinimidyl acetate and reacted at room temperature for 4 hours. Washed with 1N aqueous sodium chloride and water (0.1% SDS, 0.15 M sodium chloride, 15 mM citrate buffer), suspended in 0.2 ml, and stored at 4 ° C.

比較例1 磁性粒子バイオマグアミンヘDNAプローブを固相化した磁性粒子BM-DNAの作製:
実施例3において、磁性粒子BM-EKの代わりにバイオマグアミンを用いる以外は同様に操作して、DNAプローブ固相化磁性粒子BM-DNAを得た。
Comparative Example 1 Preparation of magnetic particle BM-DNA in which a magnetic probe biomagamine DNA probe is immobilized:
In Example 3, the same operation was performed except that biomagamine was used in place of the magnetic particle BM-EK to obtain a DNA probe-immobilized magnetic particle BM-DNA.

試験例2 磁性粒子BM-EK-DNA(実施例3)と磁性粒子BM-DNA(比較例1)の核酸捕獲能力の比較:
実施例3及び比較例1で磁性粒子に固定化したDNAプローブAに相補的でかつその5′末端にアルカリフォスファターゼを結合させたAP-プローブBをハイブリダイゼーションバッファー〔0.5%ブロッキング試薬(ベーリンガー社製),0.05%アジ化ナトリウム,0.48M塩化ナトリウム,0.048Mクエン酸三ナトリウム〕に0.05μg/mlになるように調整した。実施例3及び比較例1で作製した磁性粒子のそれぞれ10μgに溶液0.1mlを加え、53℃で15分間インキュベーションし、室温で10分間冷却した。磁性粒子を(0.1%SDS,0.015M塩化ナトリウム,0.0015Mクエン酸三ナトリウム)で2回、(0.015M塩化ナトリウム,0.0015Mクエン酸三ナトリウム)で2回洗浄した後、基質溶液(10mMパラニトロフェニルリン酸ナトリウム,25mM塩化マグネシウム,1Mジエタノールアミン−塩酸バッファーpH9.8)を0.2ml加えて37℃で30分間インキュベーションした。その後、磁性粒子を磁石で分離し、上清の100μlをマイクロタイタープレートウエルに移して、イムノリーダーで405nmの波長の吸光度を測定した。この結果を表2に示す。
Test Example 2 Comparison of nucleic acid capture ability of magnetic particle BM-EK-DNA (Example 3) and magnetic particle BM-DNA (Comparative Example 1):
AP-probe B complementary to DNA probe A immobilized on magnetic particles in Example 3 and Comparative Example 1 and having alkaline phosphatase bound to its 5 'end was mixed with a hybridization buffer [0.5% blocking reagent (Boehringer). ), 0.05% sodium azide, 0.48 M sodium chloride, 0.048 M trisodium citrate] to 0.05 μg / ml. 0.1 ml of the solution was added to 10 μg of each of the magnetic particles prepared in Example 3 and Comparative Example 1, incubated at 53 ° C. for 15 minutes, and cooled at room temperature for 10 minutes. After washing the magnetic particles twice with (0.1% SDS, 0.015 M sodium chloride, 0.0015 M trisodium citrate) and twice with (0.015 M sodium chloride, 0.0015 M trisodium citrate), the substrate solution (10 mM paranitro 0.2 ml of sodium phenylphosphate, 25 mM magnesium chloride, 1M diethanolamine-hydrochloric acid buffer (pH 9.8) was added and incubated at 37 ° C. for 30 minutes. Thereafter, the magnetic particles were separated with a magnet, 100 μl of the supernatant was transferred to a microtiter plate well, and the absorbance at a wavelength of 405 nm was measured with an immunoreader. The results are shown in Table 2.

Figure 2008134259
Figure 2008134259

表2より、実施例3の磁性粒子は比較例1の磁性粒子よりも多くのDNAプローブAが固定化されており、核酸の捕獲能力に優れていることが確認された。   From Table 2, it was confirmed that the magnetic particles of Example 3 had more DNA probes A immobilized thereon than the magnetic particles of Comparative Example 1, and were excellent in nucleic acid capturing ability.

実施例4 磁性粒子M450ヘアミノ基を導入した磁性粒子M450Aの作製:
ダイナビーズ磁性粒子M450(Uncoated,官能基は水酸基,ダイナテック社製)0.5mgをメタノール2.7mlに懸濁し、3-アミノプロピルトリエトキシシラン0.3mlを加えて65℃で2時間反応させることによりアミノ基を導入した。磁性粒子を水及び0.1%SDSで洗浄し、(0.1%SDS,0.15M塩化ナトリウム,15mMクエン酸バッファー)0.2mlに懸濁し、4℃で保存した。
Example 4 Production of Magnetic Particle M450A Introducing Amino Group into Magnetic Particle M450:
Dynabead magnetic particles M450 (Uncoated, functional group is hydroxyl group, manufactured by Dynatech) 0.5 mg is suspended in 2.7 ml of methanol, and 0.3 ml of 3-aminopropyltriethoxysilane is added and reacted at 65 ° C. for 2 hours. A group was introduced. The magnetic particles were washed with water and 0.1% SDS, suspended in 0.2 ml (0.1% SDS, 0.15 M sodium chloride, 15 mM citrate buffer) and stored at 4 ° C.

実施例5 磁性粒子M450Aヘポリグルタミン酸を結合させた磁性粒子M450A-Eの作製:
実施例1において、バイオマグアミンの代わりに実施例4で作製した磁性粒子M450Aを用いる以外は同様に操作してポリグルタミン酸を結合させ、ポリグルタミン酸結合磁性粒子M450A-Eを得た。
Example 5 Preparation of magnetic particles M450A-E to which polyglutamic acid was bound to magnetic particles M450A:
In Example 1, polyglutamic acid was bound in the same manner except that the magnetic particle M450A prepared in Example 4 was used instead of biomagamine to obtain polyglutamic acid-bound magnetic particles M450A-E.

実施例6 磁性粒子M450A-Eヘポリリジンを結合させた磁性粒子M450A-EKの作製:
実施例2において、磁性粒子BM-Eの代わりに実施例5で作製したポリグルタミン酸結合磁性粒子M450A-Eを用いる以外は同様に操作してポリリジンを結合させ、ポリグルタミン酸−ポリリジン結合磁性粒子M450A-EKを得た。
Example 6 Preparation of magnetic particles M450A-EK to which magnetic particles M450A-E and polylysine were bound:
In Example 2, polylysine was bonded in the same manner except that the polyglutamic acid-bonded magnetic particle M450A-E prepared in Example 5 was used instead of the magnetic particle BM-E, and polylysine acid-polylysine-bonded magnetic particle M450A- Got EK.

実施例7 磁性粒子M450A-EKへポリリジンを結合させた磁性粒子M450A-EKKの作製:
実施例6で作製した磁性粒子M450A-EK 5mgを100mMリン酸バッファー(pH7.8)1.5mlに懸濁し、無水コハク酸15mlを無水DMF 0.1mlに溶解したものを加えて室温で2時間撹拌した。磁性粒子を1M塩化ナトリウム水及び水で洗浄した。この磁性粒子に実施例2と同様の操作を行って更にポリリジンを結合させ、ポリグルタミン酸−ポリリジン−ポリリジン結合磁性粒子M450A-EKKを得た。
Example 7 Production of magnetic particles M450A-EKK in which polylysine was bound to magnetic particles M450A-EK:
5 mg of magnetic particles M450A-EK prepared in Example 6 were suspended in 1.5 ml of 100 mM phosphate buffer (pH 7.8), and 15 ml of succinic anhydride dissolved in 0.1 ml of anhydrous DMF was added and stirred at room temperature for 2 hours. . The magnetic particles were washed with 1M sodium chloride water and water. This magnetic particle was subjected to the same operation as in Example 2 to further bind polylysine to obtain a polyglutamic acid-polylysine-polylysine-bonded magnetic particle M450A-EKK.

実施例8 磁性粒子M450A-EKKへDNAプローブを固相化した磁性粒子M450A-EKK-DNAの作製:
実施例3において、磁性粒子BM-EKの代わりに実施例7で作製した磁性粒子M450A-EKKを用いる以外は同様に操作し、DNAプローブ固相化磁性粒子M450A-EKK-DNAを得た。
Example 8 Production of magnetic particles M450A-EKK-DNA in which a DNA probe was immobilized on magnetic particles M450A-EKK:
In Example 3, the same operation was performed except that the magnetic particle M450A-EKK prepared in Example 7 was used instead of the magnetic particle BM-EK, to obtain a DNA probe solid-phased magnetic particle M450A-EKK-DNA.

比較例2 磁性粒子M450AへDNAプローブを固相化した磁性粒子M450A-DNAの作製:
実施例3において、磁性粒子BM-EKの代わりに実施例4で作製した磁性粒子M450Aを用いる以外は同様に操作し、DNAプローブ固相化磁性粒子M450A-DNAを得た。
Comparative Example 2 Preparation of magnetic particle M450A-DNA in which a DNA probe is immobilized on magnetic particle M450A:
In Example 3, the same operation was performed except that the magnetic particle M450A prepared in Example 4 was used instead of the magnetic particle BM-EK, to obtain a DNA probe solid-phased magnetic particle M450A-DNA.

試験例3 M450A-DNA(比較例2)と磁性粒子M450A-EKK-DNA(実施例8)の核酸捕獲能力の比較:
実施例8で作製した磁性粒子M450A-EKK-DNAと比較例2で作製した磁性粒子M450A-DNAを試験例2と同様にして比較した。この結果を表3に示す。
Test Example 3 Comparison of nucleic acid capture ability between M450A-DNA (Comparative Example 2) and magnetic particles M450A-EKK-DNA (Example 8):
The magnetic particle M450A-EKK-DNA produced in Example 8 and the magnetic particle M450A-DNA produced in Comparative Example 2 were compared in the same manner as in Test Example 2. The results are shown in Table 3.

Figure 2008134259
Figure 2008134259

表3より、実施例8の磁性粒子は比較例2の磁性粒子よりも格段に多くのDNAプローブが固定化され、核酸捕獲能力に優れていることが確認された。   From Table 3, it was confirmed that the magnetic particles of Example 8 had much more DNA probes immobilized than the magnetic particles of Comparative Example 2, and were excellent in nucleic acid capturing ability.

実施例9 磁性粒子CM-MPヘポリリジンを結合した磁性粒子CMMP-Kの作製:
実施例2において、磁性粒子BM-Eの代わりに磁性粒子CM-MP(官能基はカルボキシル基,セラダイン社製)を用いる以外は同様に操作してポリリジンを結合させ、ポリリジン結合磁性粒子CMMP-Kを得た。
Example 9 Preparation of magnetic particle CMMP-K bound with magnetic particle CM-MP hepolylysine:
In Example 2, polylysine was bonded in the same manner except that magnetic particle CM-MP (functional group is carboxyl group, manufactured by Ceradyne) was used instead of magnetic particle BM-E, and polylysine-bonded magnetic particle CMMP-K was used. Got.

実施例10 磁性粒子CMMP-Kヘポリグルタミン酸を結合した磁性粒子CMMP-KEの作製:
実施例1において、バイオマグアミンの代わりに実施例9で作製したポリリジン結合磁性粒子CMMP-Kを用いる以外は同様に操作してポリグルタミン酸を結合させ、ポリリジン−ポリグルタミン酸結合磁性粒子CMMP-KEを得た。
Example 10 Preparation of magnetic particles CMMP-KE to which magnetic particles CMMP-K hepolyglutamic acid was bound:
In Example 1, polyglutamic acid was bound in the same manner except that polylysine-bound magnetic particles CMMP-K prepared in Example 9 were used instead of biomagamine, and polylysine-polyglutamic acid-bound magnetic particles CMMP-KE were combined. Obtained.

実施例11 磁性粒子CMMP-KEヘポリリジンを結合した磁性粒子CMMP-KEKの作製:
実施例2において、磁性粒子BM-Eの代わりに実施例10で作製したポリリジン−ポリグルタミン酸結合磁性粒子CMMP-KEを用いる以外は同様に操作してポリリジンを結合させ、ポリリジン−ポリグルタミン酸−ポリリジン結合磁性粒子CMMP-KEKを得た。
Example 11 Production of magnetic particles CMMP-KEK bonded with magnetic particles CMMP-KE and polylysine:
In Example 2, polylysine was bound in the same manner except that the polylysine-polyglutamic acid-bonded magnetic particle CMMP-KE prepared in Example 10 was used instead of the magnetic particle BM-E, and polylysine-polyglutamic acid-polylysine bond was bound. Magnetic particles CMMP-KEK were obtained.

実施例12 磁性粒子CMMP-KEKへDNAプローブを固相化した磁性粒子CMMP-KEK-DNAの作製:
実施例3において、磁性粒子BM-EKの代わりに実施例11で作製した磁性粒子CMMP-KEKを用いる以外は同様に操作し、DNAプローブ固相化磁性粒子CMMP-KEK-DNAを得た。
Example 12 Preparation of magnetic particle CMMP-KEK-DNA in which a DNA probe is immobilized on magnetic particle CMMP-KEK:
In Example 3, the same operation was performed except that the magnetic particle CMMP-KEK prepared in Example 11 was used instead of the magnetic particle BM-EK, to obtain a DNA probe-immobilized magnetic particle CMMP-KEK-DNA.

比較例3 磁性粒子CM-MPへDNAプローブを固相化した磁性粒子CMMP-DNAの作製:
反応容器に磁性粒子CM-MP(セラダイン社製)10mgを100mM 2-(N-モルホリノ)エタンスルホン酸バッファー(pH6.1,MESバッファー)5mlに懸濁し、磁石で分離した後、液相を除去することによって洗浄した。この操作を2回繰り返した後、100mM N-ヒドロキシサクシンイミドバッファー(pH6.1,HOSuバッファー)10mlに懸濁して、EDC 400mgを加え、室温で30分振盪して、磁性粒子を水で洗浄した。更に、100mMリン酸バッファー(pH7.8)5mlに懸濁し、これに実施例3で用いたDNAプローブA、0.625ODを加えて4時間振盪した。磁性粒子を1M塩化ナトリウム水及び水で洗浄し、(0.1%SDS,0.15M塩化ナトリウム,15Mクエン酸バッファー)0.5mlに懸濁し、4℃で保存した。
Comparative Example 3 Preparation of magnetic particle CMMP-DNA in which a DNA probe is immobilized on magnetic particle CM-MP:
10 mg of magnetic particles CM-MP (manufactured by Ceradyne) is suspended in 5 ml of 100 mM 2- (N-morpholino) ethanesulfonic acid buffer (pH 6.1, MES buffer) in a reaction vessel and separated with a magnet, and then the liquid phase is removed. By washing. After repeating this operation twice, suspended in 10 ml of 100 mM N-hydroxysuccinimide buffer (pH 6.1, HOSu buffer), added 400 mg of EDC, shaken at room temperature for 30 minutes, and washed the magnetic particles with water. . Further, the suspension was suspended in 5 ml of 100 mM phosphate buffer (pH 7.8), and the DNA probe A and 0.625OD used in Example 3 were added thereto, followed by shaking for 4 hours. The magnetic particles were washed with 1 M sodium chloride water and water, suspended in 0.5 ml (0.1% SDS, 0.15 M sodium chloride, 15 M citrate buffer) and stored at 4 ° C.

試験例4 磁性粒子CMMP-DNA(比較例3)及び磁性粒子CMMP-KEK-DNA(実施例12)を用いたWT1mRNAの測定結果の比較:
比較例3の磁性粒子CMMP-DNAを用いて癌抑制遺伝子WT1mRNAの測定を行った。測定方法は、クオンティプレックスHCV-RNA測定キット(カイロン社製)の手法に従って行った。WT1mRNAはRnessy Total RNA Kit(QIAVEN社製)を用いてヒト白血病細胞株(K562)から抽出し、PBSで希釈して検体とした。抽出緩衝液、増幅プローブ希釈液、標識プローブ希釈液、増幅プローブ、標識プローブ、基質液、Wash A及びWash BはクオンティプレックスHCV-RNA測定キットのものを用いた。また、キット中の特異プローブA及び特異プローブBは、WT1mRNAの一部に相補的なものを合成して調製した。反応用容器として、ダイナテックラボラトリーズ社のマイクロライン1を用いた。抽出緩衝液4.6ml、酵素液350μl、特異プローブA 2.8μl及び特異プローブB 2.8μlを混合し、100μlを4μg/10μlのWT1mRNAに加え、53℃で16時間インキュベーションした。更に、比較例3の磁性粒子20μgを抽出緩衝液20μlに懸濁したものを加え、53℃で4.5時間インキュベーションした。更に室温で10分間放置し、磁気分離を行い、上清を除いた。Wash Bで2回洗浄した後、増幅プローブ希釈液5.6mlと増幅プローブ40μlを混合したものを100μl加えて53℃で30分インキュベーションした。室温で10分間冷却した後、磁気分離を行い、Wash A 200μlで洗浄した後、標識プローブ希釈液5.6mlと標識プローブ32μlを混合したもの100μlを加えて53℃で15分間インキュベーションして、室温で10分間放置した。磁気分離を行い、Wash A及びWash Bでそれぞれ3回ずつ洗浄した後、基質液100μlを加え、ルミノメーターQ-1000で発光量を測定した。
また、試験する磁性粒子を実施例12のもの10μgに変えて、同様の試験を行った。発光量の測定結果を表4に示す。
Test Example 4 Comparison of WT1 mRNA measurement results using magnetic particle CMMP-DNA (Comparative Example 3) and magnetic particle CMMP-KEK-DNA (Example 12):
The tumor suppressor gene WT1 mRNA was measured using the magnetic particle CMMP-DNA of Comparative Example 3. The measurement method was performed according to the method of the Quantiplex HCV-RNA measurement kit (manufactured by Chiron). WT1 mRNA was extracted from a human leukemia cell line (K562) using Rnessy Total RNA Kit (manufactured by QIAVEN) and diluted with PBS to prepare a sample. The extraction buffer, the amplification probe dilution, the labeled probe dilution, the amplification probe, the label probe, the substrate solution, Wash A and Wash B were from the Quantitplex HCV-RNA measurement kit. Moreover, the specific probe A and the specific probe B in the kit were prepared by synthesizing a probe complementary to a part of the WT1 mRNA. As a reaction vessel, Dynaline Laboratories Microline 1 was used. 4.6 ml of extraction buffer, 350 μl of enzyme solution, 2.8 μl of specific probe A and 2.8 μl of specific probe B were mixed, 100 μl was added to 4 μg / 10 μl of WT1 mRNA, and incubated at 53 ° C. for 16 hours. Further, 20 μg of the magnetic particles of Comparative Example 3 suspended in 20 μl of extraction buffer were added and incubated at 53 ° C. for 4.5 hours. Furthermore, it was left to stand at room temperature for 10 minutes, magnetic separation was performed, and the supernatant was removed. After washing twice with Wash B, 100 μl of a mixture of 5.6 ml of amplification probe dilution and 40 μl of amplification probe was added and incubated at 53 ° C. for 30 minutes. After cooling at room temperature for 10 minutes, perform magnetic separation, wash with 200 μl Wash A, add 100 μl of a mixture of 5.6 ml of labeled probe dilution and 32 μl of labeled probe, and incubate for 15 minutes at 53 ° C. Left for 10 minutes. After magnetic separation and washing with Wash A and Wash B three times, 100 μl of substrate solution was added, and the amount of luminescence was measured with a luminometer Q-1000.
Further, the same test was performed by changing the magnetic particles to be tested to 10 μg of Example 12. Table 4 shows the measurement results of the light emission amount.

Figure 2008134259
Figure 2008134259

この結果から、表面官能基のカルボキシル基に直接DNA固定化した比較例3の磁性粒子よりも、ポリアミノ酸をコーティングし、磁性粒子の官能基をアミノ基に変換した実施例12の磁性粒子を使用した方が感度が向上していることが確認された。   From this result, the magnetic particles of Example 12 in which the polyamino acid was coated and the functional groups of the magnetic particles were converted to amino groups were used rather than the magnetic particles of Comparative Example 3 in which DNA was directly immobilized on the carboxyl group of the surface functional group. It was confirmed that the sensitivity was improved.

Claims (1)

表面にアミド結合を介してポリ酸性アミノ酸又はポリ塩基性アミノ酸が結合してなる核酸固定用磁性粒子。A magnetic particle for immobilizing nucleic acid, wherein a polyacidic amino acid or a polybasic amino acid is bonded to the surface via an amide bond.
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JPH02501753A (en) * 1987-10-26 1990-06-14 デイド、インターナショナル、インコーポレイテッド Manufacturing method of magnetically responsive polymer particles and its applications
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Publication number Priority date Publication date Assignee Title
WO2019048333A1 (en) * 2017-09-11 2019-03-14 Life Technologies As Methods and compositions for coupling nucleic acid to a functionalized support
CN111094318A (en) * 2017-09-11 2020-05-01 生命技术股份公司 Methods and compositions for coupling nucleic acids to functionalized supports
US11555183B2 (en) 2017-09-11 2023-01-17 Life Technologies Corporation Methods and compositions for coupling nucleic acid to a functionalized support
CN111094318B (en) * 2017-09-11 2024-01-09 生命技术股份公司 Methods and compositions for coupling nucleic acids to functionalized supports

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