JPH07140146A - Stable peroxidase composition and stable antibody composition - Google Patents
Stable peroxidase composition and stable antibody compositionInfo
- Publication number
- JPH07140146A JPH07140146A JP5286981A JP28698193A JPH07140146A JP H07140146 A JPH07140146 A JP H07140146A JP 5286981 A JP5286981 A JP 5286981A JP 28698193 A JP28698193 A JP 28698193A JP H07140146 A JPH07140146 A JP H07140146A
- Authority
- JP
- Japan
- Prior art keywords
- peroxidase
- antibody
- composition
- hydroxyphenyl
- activity
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Pending
Links
Classifications
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y02—TECHNOLOGIES OR APPLICATIONS FOR MITIGATION OR ADAPTATION AGAINST CLIMATE CHANGE
- Y02P—CLIMATE CHANGE MITIGATION TECHNOLOGIES IN THE PRODUCTION OR PROCESSING OF GOODS
- Y02P20/00—Technologies relating to chemical industry
- Y02P20/50—Improvements relating to the production of bulk chemicals
- Y02P20/52—Improvements relating to the production of bulk chemicals using catalysts, e.g. selective catalysts
Abstract
Description
【0001】[0001]
【産業上の利用分野】本発明は免疫学的測定に用いるペ
ルオキシダーゼ又は抗体の保存安定化に関する。BACKGROUND OF THE INVENTION 1. Field of the Invention The present invention relates to storage stabilization of peroxidase or antibody used for immunoassay.
【0002】[0002]
【従来の技術】近年、臨床検査、診断分野において、免
疫反応、酵素反応を利用した測定法が広く行われてきて
いる。2. Description of the Related Art In recent years, measuring methods using immunoreactions and enzyme reactions have been widely used in the fields of clinical examination and diagnosis.
【0003】ペルオキシダーゼは、過酸化水素を水素受
容体として種々の物質を酸化する反応を触媒する酵素で
あり、色原体を酸化し色素に変換する呈色反応に利用で
きる事から、たとえば目的生体成分に対応酸化酵素を反
応させ生成する過酸化水素を酵素反応により検出する測
定に用いられたり、酵素免疫測定法における標識酵素と
して用いられるなど、近年その重要性が増大してきてい
る。しかしながらペルオキシダーゼは溶液状態における
安定性に乏しく、室温での長時間保存においてその活性
を維持する事が極めて困難である。また、凍結乾燥を行
った場合も、ペルオキシダーゼ活性が相当低下する事が
知られている。Peroxidase is an enzyme that catalyzes a reaction of oxidizing various substances by using hydrogen peroxide as a hydrogen acceptor, and can be used for a color reaction for oxidizing a chromogen and converting it into a dye, and therefore, for example, a target organism. In recent years, its importance has been increasing, for example, it is used for measurement in which hydrogen peroxide produced by reacting a component with a corresponding oxidase is detected by an enzymatic reaction, or as a labeling enzyme in an enzyme immunoassay. However, peroxidase has poor stability in a solution state, and it is extremely difficult to maintain its activity during long-term storage at room temperature. It is also known that the peroxidase activity is considerably reduced even when freeze-dried.
【0004】また、免疫測定に用いる抗体も、特に低濃
度の場合、経時的に活性が低下する事が知られている。
また、この傾向は、溶液の温度が高いほど著しい。It is also known that the antibodies used for immunoassays decrease in activity over time, especially at low concentrations.
Further, this tendency becomes more remarkable as the temperature of the solution increases.
【0005】それ故、ペルオキシダーゼ及び抗体は長期
保存が難しく、これらを測定用試薬もしくは診断用試薬
として使用するには品質保証の点からも不充分なもので
あり、その安定化が強く要望されていた。また、特に、
ペルオキシダーゼと抗体とが結合したペルオキシダーゼ
標識抗体を使用する診断用試薬の場合、一方の安定化が
他方の活性を阻害することがないように、ペルオキシダ
ーゼ及び抗体を同一方法で同時に安定化する事が最も強
く望まれていた。Therefore, it is difficult to store peroxidase and antibody for a long period of time, and it is insufficient from the viewpoint of quality assurance to use them as measuring reagents or diagnostic reagents, and there is a strong demand for their stabilization. It was Also, especially
In the case of a diagnostic reagent that uses a peroxidase-labeled antibody in which a peroxidase and an antibody are bound, it is most preferable to simultaneously stabilize the peroxidase and the antibody by the same method so that the stabilization of one does not inhibit the activity of the other. It was strongly desired.
【0006】ペルオキシダーゼ又は抗体の安定化する試
みとして従来から知られた方法に、例えば、特開昭59-2
5683号記載のポリアルキレングリコールを添加する方
法、特開昭60-188067号記載の糖又は糖アルコールを添
加する方法、或いは特開平2-72982号記載の水酸基とア
ミド基を同時に有するベンゼン誘導体を添加する方法な
どが知られているが、安定化には未だ不十分であり、そ
の改良が探索されている。A method known in the prior art as an attempt to stabilize peroxidase or antibody is disclosed in, for example, JP-A-59-2.
A method of adding a polyalkylene glycol described in 5683, a method of adding a sugar or a sugar alcohol described in JP-A-60-188067, or a benzene derivative having simultaneously a hydroxyl group and an amide group described in JP-A-2-72982. Although a method of doing so is known, it is still insufficient for stabilization, and its improvement is being sought.
【0007】[0007]
【発明が解決しようとする課題】前記の状況に照し、本
発明の第1の目的は安定化されたペルオキシダーゼを含
有するペルオキシダーゼ組成物を提供する事であり、ま
た、第2の目的は安定化された抗体を含有する抗体組成
物を提供する事である。In view of the above situation, a first object of the present invention is to provide a peroxidase composition containing a stabilized peroxidase, and a second object thereof is to stabilize the composition. It is intended to provide an antibody composition containing a modified antibody.
【0008】[0008]
【課題を解決するための手段】本発明者らはペルオキシ
ダーゼ及び抗体の活性低下を抑制する方法を鋭意検討し
た結果、ペルオキシダーゼと、ヒドロキシフェニル−ア
ルコキシシランよりなるペルオキシダーゼ組成物、又ヒ
ドロキシフェニル−アルコキシシランを添加することに
よるペルオキシダーゼの安定化方法により達成されるこ
とを見出した。Means for Solving the Problems As a result of intensive investigations by the present inventors on a method for suppressing the activity reduction of peroxidase and antibody, a peroxidase composition comprising peroxidase and hydroxyphenyl-alkoxysilane, and hydroxyphenyl-alkoxysilane. It was found that this was achieved by a method of stabilizing peroxidase by adding
【0009】別の態様として、抗体と、ヒドロキシフェ
ニル−アルコキシシランを含む抗体組成物又は、ヒドロ
キシフェニル−アルコキシシランを添加することによる
抗体の安定化方法により上記目的は達成される。As another embodiment, the above object is achieved by an antibody composition containing an antibody and hydroxyphenyl-alkoxysilane or a method for stabilizing an antibody by adding hydroxyphenyl-alkoxysilane.
【0010】好ましくは、ヒドロキシフェニル−アルコ
キシシランが、下記一般式(1)で示される化合物であ
るが、より好ましくは、p−又はo−ヒドロキシフェニ
ル−アルコキシシランである。The hydroxyphenyl-alkoxysilane is preferably a compound represented by the following general formula (1), and more preferably p- or o-hydroxyphenyl-alkoxysilane.
【0011】[0011]
【化3】 [Chemical 3]
【0012】式中、R1、R2及びR3は炭素数5以下の
低級アルキル基を表し、各々は置換基を有してもよい。
更に、好ましくはアルキル基がメチル基、若しくはエチ
ル基である。In the formula, R 1 , R 2 and R 3 represent a lower alkyl group having 5 or less carbon atoms, each of which may have a substituent.
Furthermore, the alkyl group is preferably a methyl group or an ethyl group.
【0013】また、フェニル基が置換基を有していても
良い。Further, the phenyl group may have a substituent.
【0014】一般式(1)で示される化合物は、例えば o-ヒドロキシフェニルトリメトキシシラン o-ヒドロキシフェニルトリエトキシシラン o-ヒドロキシフェニルトリブトキシシラン p-ヒドロキシフェニルトリメトキシシラン p-ヒドロキシフェニルトリエトキシシラン p-ヒドロキシフェニルトリブトキシシラン o-ヒドロキシフェニルジメトキシエトキシシラン o-ヒドロキシフェニルジエトキシメトキシシラン o-ヒドロキシフェニルジメトキシブトキシシラン p-ヒドロキシフェニルジメトキシエトキシシラン p-ヒドロキシフェニルジエトキシメトキシシラン p-ヒドロキシフェニルジメトキシブトキシシラン o-ヒドロキシフェニルトリプロポキシシラン p-ヒドロキシフェニルトリプロポキシシラン などが挙げられ、好ましくはp-又はo-ヒドロキシフェニ
ルトリメトキシシランである。これらの化合物は、0.03
mM濃度以上好ましくは0.3mM以上、より好ましくは1〜
3mM濃度添加される。The compound represented by the general formula (1) is, for example, o-hydroxyphenyltrimethoxysilane o-hydroxyphenyltriethoxysilane o-hydroxyphenyltributoxysilane p-hydroxyphenyltrimethoxysilane p-hydroxyphenyltriethoxysilane. p-hydroxyphenyltributoxysilane o-hydroxyphenyldimethoxyethoxysilane o-hydroxyphenyldiethoxymethoxysilane o-hydroxyphenyldimethoxybutoxysilane p-hydroxyphenyldimethoxyethoxysilane p-hydroxyphenyldiethoxymethoxysilane p-hydroxyphenyldimethoxybutoxysilane Silanes such as o-hydroxyphenyltripropoxysilane and p-hydroxyphenyltripropoxysilane are preferred, and p- or o-hydroxy is preferred. It is E sulfonyl trimethoxysilane. These compounds have 0.03
mM concentration or higher, preferably 0.3 mM or higher, more preferably 1 to
3 mM concentration is added.
【0015】本発明に係るペルオキシダーゼとしては植
物由来、動物由来、微生物由来等、いずれの由来のもの
でもよい。その例としてはホースラデッシュペルオキシ
ダーゼ、ラクトペルオキシダーゼ、グルタチオンペルオ
キシダーゼ、ミエロペルオキシダーゼ、チトクロームC
ペルオキシダーゼ等が挙げられるが、特にホースラデッ
シュペルオキシダーゼが好ましい。The peroxidase according to the present invention may be derived from any of plant origin, animal origin, microorganism origin and the like. Examples thereof are horseradish peroxidase, lactoperoxidase, glutathione peroxidase, myeloperoxidase, cytochrome C.
Examples thereof include peroxidase, but horseradish peroxidase is particularly preferable.
【0016】本発明に係るペルオキシダーゼは非結合型
の単体でも良く、また他の有用物質との結合体でも良
い。また、ペルオキシダーゼと抗ペルオキシダーゼ抗体
より成る複合体であっても良い。The peroxidase according to the present invention may be a non-bonding simple substance, or may be a conjugate with another useful substance. It may also be a complex composed of peroxidase and anti-peroxidase antibody.
【0017】本発明に係るペルオキシダーゼの結合体と
してはペルオキシダーゼが他の有用な物質と結合したも
のであれば特に限定されないが、免疫活性物質との結合
体が好ましい。免疫活性物質としては、抗原、抗体、ハ
プテン、プロティンAなどが挙げられる。抗原もしくは
ハプテンとしては、たとえば蛋白質、糖質、脂質、複合
糖質、多糖類、核酸、酵素、ホルモン、ハプテン、抗生
物質、細菌抗原、ウイルス抗原、癌抗原、アビジン、ビ
オチン等が挙げられる。本発明の第2の形態に係る抗体
又はペルオキシダーゼと結合可能な抗体としては、前記
抗原もしくはハプテンを従来既知の方法でウサギ、ヤ
ギ、マウス等の哺乳動物やニワトリ等の鳥類に免疫する
事によりその血清中から得られる抗体や、細胞融合等に
より作製させたハイブリドーマやウイルスにより癌化さ
せた形質細胞から得られるモノクローナル抗体が挙げら
れ、またこれらの断片、例えばFab,F(ab′)2等も含まれ
る。The peroxidase conjugate according to the present invention is not particularly limited as long as it is a conjugate of peroxidase with other useful substances, but a conjugate with an immunoactive substance is preferable. Examples of the immunologically active substance include antigens, antibodies, haptens, protein A and the like. Examples of the antigen or hapten include proteins, sugars, lipids, glycoconjugates, polysaccharides, nucleic acids, enzymes, hormones, haptens, antibiotics, bacterial antigens, virus antigens, cancer antigens, avidin, biotin and the like. The antibody according to the second aspect of the present invention or the antibody capable of binding to peroxidase is prepared by immunizing a mammal such as rabbit, goat, mouse or the like or a bird such as chicken by immunizing the antigen or hapten by a conventionally known method. Antibodies obtained from serum, and monoclonal antibodies obtained from plasma cells transformed by hybridomas and viruses produced by cell fusion and the like, and also fragments thereof, such as Fab, F (ab ') 2 etc. included.
【0018】本発明の第2の形態に係る抗体はそれを用
いる測定に有用な物質、たとえば標識物質や免疫活性物
質と結合していても良い。標識物質としてはラジオアイ
ソトープ、ペルオキシダーゼ、アルカリフォスファター
ゼ、β-ガラクトシダーゼ等の酵素、蛍光物質、発光物
質、ビオチン、アビジン、キレート、金属コロイド、毒
素等が挙げられ免疫活性物質としては、たとえば抗原、
抗体、ハプテン等が挙げられる。The antibody according to the second aspect of the present invention may be bound to a substance useful for measurement using the same, for example, a labeling substance or an immunoactive substance. Examples of the labeling substance include radioisotopes, peroxidase, alkaline phosphatase, enzymes such as β-galactosidase, fluorescent substances, luminescent substances, biotin, avidin, chelates, metal colloids, and toxins.
Examples include antibodies and haptens.
【0019】ペルオキシダーゼと有用な物質との結合も
しくは抗体と有用な物質との結合は吸着等の物理的結合
やイオン結合、共有結合等の化学的結合などいずれでも
よく、共有結合が好ましい。その結合の方法としては種
々の公知の方法に従えばよく、たとえばグルタルアルデ
ヒドを架橋剤として用いアミノ基とアミノ基を結合させ
る方法やペルオキシダーゼの糖鎖の過沃素酸処理により
生成させたアルデヒド基と物質のアミノ基を結合させる
方法などが例として挙げられる。The binding between peroxidase and a useful substance or the binding between an antibody and a useful substance may be a physical bond such as adsorption, an ionic bond, a chemical bond such as a covalent bond, and a covalent bond is preferred. As a method of binding, various known methods may be used, for example, a method of binding an amino group and an amino group using glutaraldehyde as a cross-linking agent or an aldehyde group formed by treatment of a sugar chain of peroxidase with a periodic acid. Examples include a method of binding an amino group of a substance.
【0020】本発明の組成物にはその効果を高めるため
動物血清、たとえば馬血清、牛血清、羊血清、兎血清、
人血清や血清成分、たとえば牛アルブミン、ヒトアルブ
ミン等と含有させる事が好ましく、溶液状組成物の場
合、その含有量は血清ならば1〜50(w/v)%、血清成分
ならば0.1〜5(W/V)%が好ましい。In order to enhance the effect of the composition of the present invention, animal serum such as horse serum, bovine serum, sheep serum, rabbit serum,
Human serum or serum components, for example, bovine albumin, human albumin, etc. are preferably contained. In the case of a solution composition, the content is 1 to 50 ( w / v )% for serum and 0.1 to 10 for serum components. 5 ( W / V )% is preferred.
【0021】また、必要ならば他の物質、たとえば、ゼ
ラチン、卵白アルブミン、カゼイン等の蛋白質や、ポリ
アルキレングリコール等の水溶性高分子、蔗糖等の糖
類、チメロザール等の防腐剤などを含有しても良い。If necessary, other substances, for example, proteins such as gelatin, ovalbumin, casein, etc., water-soluble polymers such as polyalkylene glycol, saccharides such as sucrose, preservatives such as thimerosal, etc. may be contained. Is also good.
【0022】本発明の組成物は、任意の緩衝剤や塩化ナ
トリウム等の塩類を含有しても良い。緩衝剤としてはト
リス系、燐酸系、炭酸系、酢酸系等通常用いられるもの
が使用可能であり、水溶液中のpHがペルオキシダーゼ
組成物の場合は4〜9、抗体組成物の場合は3〜11を示
すものが好ましい。The composition of the present invention may contain any buffering agent and salts such as sodium chloride. As the buffering agent, a commonly used buffer such as Tris-based, phosphoric acid-based, carbonic acid-based, acetic acid-based can be used. When the pH in the aqueous solution is a peroxidase composition, it is 4 to 9, and when it is an antibody composition, it is 3 to 11 Is preferable.
【0023】溶液状組成物の調製時における各成分の添
加の順序は特に限定されるものではない。The order of adding each component at the time of preparing the solution composition is not particularly limited.
【0024】ペルオキシダーゼ活性の測定は、本発明の
ペルオキシダーゼ組成物と過酸化水素及び基質たとえば
o-フェニレンジアミン等の色原体を接触させ、その酵素
反応の程度を解析する事により行わせる。色原体を用い
た場合は生成色素の吸光度を測定する事によりその解析
は行われる。The peroxidase activity is measured by measuring the peroxidase composition of the present invention with hydrogen peroxide and a substrate such as
It is performed by contacting a chromogen such as o-phenylenediamine and analyzing the degree of the enzymatic reaction. When a chromogen is used, the analysis is performed by measuring the absorbance of the produced dye.
【0025】抗体活性の測定は一般の免疫測定法が利用
できる。たとえば、凝集法、競合法、サンドウイッチ
法、ELISA法などが可能である。一例としては被験標識
抗体と担体に固定化した対応抗原とを反応させ、担体に
結合した標識の量を測定する方法が挙げられる。A general immunoassay can be used to measure the antibody activity. For example, agglutination method, competitive method, sandwich method, ELISA method, etc. are possible. One example is a method of reacting a test labeled antibody with a corresponding antigen immobilized on a carrier and measuring the amount of the label bound to the carrier.
【0026】ペルオキシダーゼまたは抗体の活性の安定
性の評価は、たとえば経時的な活性の変化の検討や4℃
保持の場合と37℃保持の場合との活性の比較によって行
なう事ができる。The stability of the activity of peroxidase or antibody can be evaluated, for example, by examining the change in activity over time or at 4 ° C.
It can be carried out by comparing the activity between the case of holding and the case of holding at 37 ° C.
【0027】本発明のペルオキシダーゼの組成物は長期
保存、室温保存及び凍結乾燥時におけるペルオキシダー
ゼの活性が保持される。また、本発明の抗体組成物も同
様に保存安定性に優れる。本発明に係る置換ベンゼン環
は、ペルオキシダーゼ及び抗体の双方にとって安定剤と
して有用であるため、ペルオキシダーゼ標識抗体の安定
化剤として特に有用である。これら本発明の組成物を適
用した免疫学的測定用試薬は経時安定性に優れる事か
ら、臨床検査、診断分野において有用性が極めて高い。The peroxidase composition of the present invention retains the activity of peroxidase during long-term storage, room temperature storage and freeze-drying. Also, the antibody composition of the present invention is similarly excellent in storage stability. The substituted benzene ring according to the present invention is useful as a stabilizer for both peroxidase and antibody, and thus is particularly useful as a stabilizer for peroxidase-labeled antibody. The immunological measurement reagent to which the composition of the present invention is applied has excellent stability over time, and thus has extremely high utility in the fields of clinical examination and diagnosis.
【0028】[0028]
【実施例】以下、実施例により本発明を更に詳細に説明
する。EXAMPLES The present invention will be described in more detail below with reference to examples.
【0029】実施例1 100mMの塩化ナトリウムを含む25mM燐酸緩衝液(pH7.
4:以下PBSと略す)中に、1(W/V)%の牛血清ア
ルブミン(以下BSAと略す)及び1μg/mlのホース
ラディッシュペルオキシダーゼと、安定化剤としてp-ヒ
ドロキシフェニルトリメトキシシランまたはo-ヒドロキ
シフェニルトリメトキシシランとを溶解しペルオキシダ
ーゼ溶液を調製した。これらの溶液は4℃または37℃で
1週間保持した。なお、比較に安定化剤としてポリエチ
レングリコールもしくは蔗糖を加えたもの、及び安定化
剤を加えないものも同時に調製した。Example 1 25 mM phosphate buffer containing 100 mM sodium chloride (pH 7.
4: 1 ( W / V )% bovine serum albumin (hereinafter abbreviated as BSA) and 1 μg / ml horseradish peroxidase in p) and p-hydroxyphenyltrimethoxysilane or o as a stabilizer -Hydroxyphenyltrimethoxysilane was dissolved to prepare a peroxidase solution. These solutions were kept at 4 ° C or 37 ° C for 1 week. For comparison, polyethylene glycol or sucrose was added as a stabilizer and those without a stabilizer were also prepared at the same time.
【0030】保持したペルオキシダーゼ溶液をPBSに
て10倍に希釈しそのペルオキシダーゼ活性を以下のごと
く測定した。すなわち、2mg/mlの濃度のo-フェニレン
ジアミン及び0.02%の過酸化水素を含むクエン酸−燐酸
緩衝液(pH5.0)500μlに2μlの上記希釈溶液を加
え、37℃にて30分間反応させた後、2mlの1N硫酸を加
え、492nmの吸光度を測定することによって行った。The retained peroxidase solution was diluted 10 times with PBS and its peroxidase activity was measured as follows. That is, 2 μl of the diluted solution was added to 500 μl of a citric acid-phosphate buffer solution (pH 5.0) containing o-phenylenediamine at a concentration of 2 mg / ml and 0.02% hydrogen peroxide, and the mixture was reacted at 37 ° C. for 30 minutes. After that, 2 ml of 1N sulfuric acid was added, and the absorbance at 492 nm was measured.
【0031】調製直後のペルオキシダーゼ活性を100%
とし、1週間保持されたペルオキシダーゼ溶液のペルオ
キシダーゼ活性を表1に示す。100% of peroxidase activity immediately after preparation
Table 1 shows the peroxidase activity of the peroxidase solution retained for 1 week.
【0032】[0032]
【表1】 [Table 1]
【0033】表1から本発明の化合物を添加した試料
は、ペルオキシダーゼ活性が37℃にて少なくとも1週間
安定に保持されることが解る。It can be seen from Table 1 that the sample to which the compound of the present invention is added stably retains the peroxidase activity at 37 ° C. for at least 1 week.
【0034】実施例2 抗GATモノクローナル抗体MAb8628(特開平3-2590
93)を石川栄治 編「酵素免疫測定法(第3版)医学書
院 1987年」P108の方法にてホースラディッシュペル
オキシダーゼ標識し、標識抗体を作成した。Example 2 Anti-GAT monoclonal antibody MAb8628 (Japanese Patent Laid-Open No. 3590/1993)
93) was labeled with horseradish peroxidase by the method of P108, “Enzyme-linked immunosorbent assay (3rd edition) Medical Shoin 1987” edited by Eiji Ishikawa to prepare a labeled antibody.
【0035】この標識抗体を1%のBSAを含むPBS
にて200ng/mlとなるように希釈し、さらに表2に示す
ヒドロキシフェニル−アルコキシシランを溶解し、標識
抗体液を調製した。これらの標識抗体液は4℃または37
℃で1週間保持した。なお、比較に安定化剤として及び
ポリエチレングリコールもしくは蔗糖を加えたもの、及
び安定化剤を加えないものも同時に調製した。This labeled antibody was added to PBS containing 1% BSA.
Was diluted to 200 ng / ml, and the hydroxyphenyl-alkoxysilane shown in Table 2 was dissolved to prepare a labeled antibody solution. These labeled antibody solutions should be 4 ℃ or 37
Hold at 1 ° C for 1 week. For comparison, those with polyethylene glycol or sucrose as stabilizers and those without stabilizers were prepared at the same time.
【0036】この保持した標識抗体液を2次抗体として
用い、以下の様にしてペルオキシダーゼ安定性、抗体安
定性を算出した。Using this retained labeled antibody solution as a secondary antibody, peroxidase stability and antibody stability were calculated as follows.
【0037】ポリスチレンビーズと10μg/mlの濃度の
抗GATモノクローナル抗体MAb8513(特開平3-2590
93)をPBS中にて4℃にて1晩静置した後、1%BS
A/PBSにて37℃、1晩ブロッキングし抗体固定化ビ
ーズを調製した。GAT濃度が約50U/mlの検体(癌患
者血清)50μlを0.01%Tween−20含有PBS200μlにて
希釈し、調製した抗体固定化ビーズ1ケを加え、45℃に
て1時間反応させた。PBSにて3回洗浄後、上記標識
抗体液250μlを加え、20℃にて2時間反応させた。PB
Sにて4回洗浄後、3mg/mlの濃度のo-フェニレンジア
ミン及び0.02%の過酸化水素を含むクエン酸−燐酸緩衝
液(pH5.0)300μlを加え、室温にて30分間発色反応さ
せた。その後1mlの1N硫酸を加え、492nmの吸光度を
測定した。Polystyrene beads and anti-GAT monoclonal antibody MAb8513 at a concentration of 10 μg / ml (JP-A-3-2590)
93) in PBS overnight at 4 ° C, then 1% BS
Antibody-immobilized beads were prepared by blocking with A / PBS at 37 ° C. overnight. 50 μl of a sample (serum of cancer patient) having a GAT concentration of about 50 U / ml was diluted with 200 μl of 0.01% Tween-20-containing PBS, 1 prepared antibody-immobilized bead was added, and the mixture was reacted at 45 ° C. for 1 hour. After washing three times with PBS, 250 μl of the above-mentioned labeled antibody solution was added, and the mixture was reacted at 20 ° C. for 2 hours. PB
After washing 4 times with S, 300 μl of citric acid-phosphate buffer solution (pH 5.0) containing o-phenylenediamine at a concentration of 3 mg / ml and 0.02% hydrogen peroxide was added, and color reaction was performed at room temperature for 30 minutes. It was Thereafter, 1 ml of 1N sulfuric acid was added, and the absorbance at 492 nm was measured.
【0038】4℃保持の標識抗体を用いて、既知量のG
AT濃度を持った標準品を同様に測定して得た検量線を
用い、各種標識抗体を用いたときのGAT濃度を算定
し、4℃保持の標識抗体を用いた場合のGAT濃度に対
する37℃保持の場合のGAT濃度の割合を標識抗体安定
性とした。Using a labeled antibody kept at 4 ° C., a known amount of G
Using a calibration curve obtained by similarly measuring a standard product having an AT concentration, the GAT concentration when various labeled antibodies were used was calculated, and the temperature was 37 ° C against the GAT concentration when the labeled antibody retained at 4 ° C was used. The ratio of GAT concentration in the case of retention was defined as the labeled antibody stability.
【0039】また、標識抗体のペルオキシダーゼ活性を
実施例1と同様に測定し、4℃保持の活性に対する37℃
保持の活性をペルオキシダーゼ安定性とした。Further, the peroxidase activity of the labeled antibody was measured in the same manner as in Example 1, and the peroxidase activity at 37 ° C. relative to the activity at 4 ° C.
The activity of retention was peroxidase stability.
【0040】また、ペルオキシダーゼ安定性に対する標
識抗体安定性の割合を抗体安定性とし、結果を表2に示
す。The ratio of labeled antibody stability to peroxidase stability was defined as antibody stability, and the results are shown in Table 2.
【0041】[0041]
【表2】 [Table 2]
【0042】表2から本発明の化合物を添加した試料
は、ペルオキシダーゼ活性及び抗体活性が37℃にて少
なくとも1週間安定に保持されることが解る。From Table 2, it can be seen that the sample to which the compound of the present invention is added stably retains the peroxidase activity and the antibody activity at 37 ° C. for at least 1 week.
【0043】実施例3 実施例2で調製した標識抗体を1%のBSAを含むPB
Sにて200ng/mlとなるように希釈し、さらに表3に示
す安定化剤を溶解し、さらに馬血清や蔗糖を加え、標識
抗体液を調製した。これらの標識抗体液は0.5mlずつバ
イアル瓶に分注し、−40℃にて凍結後、減圧下に凍結乾
燥を行った。凍結乾燥終了後、純水0.5mlを加え、実施
例2と同様にペルオキシダーゼ活性とGAT濃度を得
た。安定性は凍結乾燥しなかった場合に対する凍結乾燥
した場合の割合として算出し、結果を表3に示す。Example 3 The labeled antibody prepared in Example 2 was added to PB containing 1% BSA.
The solution was diluted with S to 200 ng / ml, the stabilizers shown in Table 3 were dissolved, and horse serum and sucrose were further added to prepare a labeled antibody solution. 0.5 ml of each of these labeled antibody solutions was dispensed into vials, frozen at -40 ° C, and then freeze-dried under reduced pressure. After the freeze-drying was completed, 0.5 ml of pure water was added to obtain the peroxidase activity and GAT concentration in the same manner as in Example 2. The stability was calculated as the ratio of the case of non-lyophilized to the case of non-lyophilized, and the results are shown in Table 3.
【0044】[0044]
【表3】 [Table 3]
【0045】表3から本発明の化合物を添加した試料
は、凍結乾燥操作によるペルオキシダーゼ活性の低下を
制御する。なお、馬血清や蔗糖を共存させた場合は、そ
の効果は顕著である。また、凍結乾燥操作による抗体活
性の低下も制御する。From Table 3, the sample to which the compound of the present invention is added controls the decrease in peroxidase activity due to the freeze-drying operation. When horse serum or sucrose coexists, the effect is remarkable. It also controls the decrease in antibody activity due to the freeze-drying operation.
【0046】[0046]
【発明の効果】本発明により安定化されたペルオキシダ
ーゼを含有するペルオキシダーゼ組成物及び安定化され
た抗体を含有する抗体組成物が得られた。According to the present invention, a peroxidase composition containing a stabilized peroxidase and an antibody composition containing a stabilized antibody were obtained.
Claims (6)
ル−アルコキシシランよりなるペルオキシダーゼ組成
物。1. A peroxidase composition comprising peroxidase and hydroxyphenyl-alkoxysilane.
を添加することによるペルオキシダーゼの安定化方法。2. A method for stabilizing peroxidase by adding hydroxyphenyl-alkoxysilane.
が、下記一般式(1)で示される化合物であることを特
徴とする請求項1記載のペルオキシダーゼ組成物又は請
求項2記載のペルオキシダーゼの安定化方法。 【化1】 式中、R1、R2及びR3は炭素数5以下の低級アルキル
基を表し、各々は置換基を有してもよい。3. The peroxidase composition according to claim 1 or the method for stabilizing peroxidase according to claim 2, wherein the hydroxyphenyl-alkoxysilane is a compound represented by the following general formula (1). [Chemical 1] In the formula, R 1 , R 2 and R 3 represent a lower alkyl group having 5 or less carbon atoms, and each may have a substituent.
シシランを含む抗体組成物。4. An antibody composition comprising an antibody and hydroxyphenyl-alkoxysilane.
を添加することによる抗体の安定化方法。5. A method for stabilizing an antibody by adding hydroxyphenyl-alkoxysilane.
が、下記一般式(1)で示される化合物であることを特
徴とする請求項4記載の抗体組成物又は請求項5記載の
抗体の安定化方法。 【化2】 式中、R1、R2及びR3は炭素数5以下の低級アルキル
基を表し、各々は置換基を有してもよい。6. The antibody composition according to claim 4 or the method for stabilizing an antibody according to claim 5, wherein the hydroxyphenyl-alkoxysilane is a compound represented by the following general formula (1). [Chemical 2] In the formula, R 1 , R 2 and R 3 represent a lower alkyl group having 5 or less carbon atoms, and each may have a substituent.
Priority Applications (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP5286981A JPH07140146A (en) | 1993-11-16 | 1993-11-16 | Stable peroxidase composition and stable antibody composition |
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| JP5286981A JPH07140146A (en) | 1993-11-16 | 1993-11-16 | Stable peroxidase composition and stable antibody composition |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| JPH07140146A true JPH07140146A (en) | 1995-06-02 |
Family
ID=17711477
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| JP5286981A Pending JPH07140146A (en) | 1993-11-16 | 1993-11-16 | Stable peroxidase composition and stable antibody composition |
Country Status (1)
| Country | Link |
|---|---|
| JP (1) | JPH07140146A (en) |
Cited By (1)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2001090017A1 (en) * | 2000-05-24 | 2001-11-29 | Saint-Gobain Vetrotex France S.A. | Sizing composition for glass yarns, resulting yarns and use thereof in cement products |
-
1993
- 1993-11-16 JP JP5286981A patent/JPH07140146A/en active Pending
Cited By (3)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2001090017A1 (en) * | 2000-05-24 | 2001-11-29 | Saint-Gobain Vetrotex France S.A. | Sizing composition for glass yarns, resulting yarns and use thereof in cement products |
| FR2809389A1 (en) * | 2000-05-24 | 2001-11-30 | Vetrotex France Sa | SIZING COMPOSITION FOR GLASS WIRES, THESE WIRES AND THEIR USE IN CEMENT PRODUCTS |
| CN1298653C (en) * | 2000-05-24 | 2007-02-07 | 法国圣戈班韦特罗特斯有限公司 | Sizing composition for glass yarns, resulting yarns and use thereof in cement products |
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