CN1311053C - Intensifier for enzymatically chemical luminous reaction - Google Patents

Intensifier for enzymatically chemical luminous reaction Download PDF

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Publication number
CN1311053C
CN1311053C CN 98125659 CN98125659A CN1311053C CN 1311053 C CN1311053 C CN 1311053C CN 98125659 CN98125659 CN 98125659 CN 98125659 A CN98125659 A CN 98125659A CN 1311053 C CN1311053 C CN 1311053C
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China
Prior art keywords
intensifier
chemical luminous
measurement
toughener
enzymatically
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CN 98125659
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CN1257904A (en
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张雯艳
朱国逸
丁家华
李峰
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Changchun Institute of Applied Chemistry of CAS
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Changchun Institute of Applied Chemistry of CAS
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  • Investigating Or Analysing Materials By The Use Of Chemical Reactions (AREA)
  • Measuring Or Testing Involving Enzymes Or Micro-Organisms (AREA)

Abstract

The present invention belongs to the use of a novel intensifier for enzymatically chemical luminous reaction. Intensifier discovery can cause the development and application of an intensifier with a similar structure. Along with intensifier use, a new measurement system is provided for the measurement of horse radish peroxidase and the chemical luminous enzyme immunoassay of an enzyme labelling object of the measurement of horse radish peroxidase. The intensifier is easy to dissolve in water and is different from organic substances, such as phenol, etc., which need dissolving in an organic solvent, and the present invention has the special advantage in measurement, preservation and reagent kit development. A chemical luminous reactive system using sodium tetraphenylboron as the intensifier is used for measuring thyroxine, insulin and triiodothyronine.

Description

The novel enhanced agent of enzyme-catalyzed chemical luminescence reaction
The invention belongs to the purposes of enzyme-catalyzed chemical luminescence increased response agent.
By luminous agent, the luminescence system that oxygenant and catalyzer are formed is widely used in numerous areas for a long time always, in recent years, and along with the development of chemiluminescence immunoassay technology, based on HRP catalysis luminol,3-aminophthalic acid cyclic hydrazide-H 2O 2The chemiluminescence enzyme immunoassay technical development of chemical luminous system is very fast, but the direct catalytic sensitivity of HRP is very low, can't be used to detect the albumen and the nucleic acid of trace.Until the eighties middle and later periods, people have found that successively two classes can reach its luminous enhanced material of enhancing, just make this technology promptly be applied to genetic analysis and field of immunodetection, one class is 6-hydroxybenzothiazole and derivative thereof, some itself is exactly a fluorescent substance in the middle of them, as firefly luciferin etc.Another kind of is the phenols with para-orienting group, as to iodophenol, and p-phenyl phenol etc.The luminous effect of enhancing of this two classes material is high, does the background luminescence that the time spent occurs separately but also can reduce oxygenant and luminous agent etc. greatly, fluorescent lifetime can be extended to several hours simultaneously.Therefore they are widely applied in the immunochemiluminometry.
Britain has found the Wolfson research department that a series of compound can strengthen HRP catalysis luminol chemiluminescence, and luminous signal is stable.This achievement began to use the end of the eighties, and used toughener has fluorescein, and thiazole is to iodophenol etc.Patent: 87-251511 (Phenols asenhancers of the chemiluminescent), 90-101018 (Chemiluminescenceenhancer), very high to iodophenol enhanced chemiluminescence mensuration HRP and marker sensitivity thereof, use at most.These tougheners all have similar structure, promptly have the aromatic cycle compound of several substituted radicals.
The purpose of this invention is to provide the novel enhanced agent of enzyme-catalyzed chemical luminescence reaction.This toughener is made up of central atom boron and four phenyl ring coordinations being different from the toughener that generally adopts at present aspect structure and the characteristic.
The novel enhanced agent of enzyme-catalyzed chemical luminescence reaction provided by the invention has following basic structure:
Wherein, R=H, F, Cl, Br, I, NO 2, hydroxyl, alkyl, alkoxyl group; M=Na +, K +The sodium tetraphenylborate pure substance is a colourless crystallization, and is soluble in water and form clarifying colourless solution.Form the big π key of delocalization because it has a plurality of phenyl ring, electron transport is more prone to.Therefore used as the toughener of HRP catalysis luminol,3-aminophthalic acid cyclic hydrazide-hydrogen peroxide chemiluminescence reaction.Find that when inquiring into the enhancing luminescence mechanism of sodium tetraphenylborate what to adopt sodium tetraphenylborate be the luminescent spectrum of system of toughener and emmission spectrum with no toughener system is consistent, but change has taken place in the excitation spectrum that reacts.For relatively, also measured luminescent spectrum, emmission spectrum and the excitation spectrum of p-phenyl phenol simultaneously.
The various toughener system that existing patent report is crossed, though they are inequality fully on reinforced effects, their excitation spectrum, emmission spectrum is similar substantially with luminescent spectrum character, and this is because the mechanism of their luminous effect of enhancing is identical.Though sodium tetraphenylborate has identical feature with its luminescent spectrum of above-mentioned system and emmission spectrum, but excitation spectrum is obviously different, illustrated that its stimulated luminescence process has different courses, this is summed up as structural difference is that sodium tetraphenylboron has the big π key of conjugation that a plurality of phenyl ring form, and electron transport is more prone to.
The optimum concn of toughener sodium tetraphenylborate, the enhanced chemiluminescence effect, medium to the suitableeest luminol,3-aminophthalic acid cyclic hydrazide concentration and the concentration of hydrogen peroxide that strengthens luminous influence and luminous reaction system is: the optimum concn of sodium tetraphenylborate is between 0.1-60mmol/L, the pH value is in the 7.0-9.0 scope, and luminol,3-aminophthalic acid cyclic hydrazide concentration is 1 * 10 -3-1 * 10 -5Mmol/L, concentration of hydrogen peroxide is 10 -2-10 -4The luminous maximum that obtains during mmol/L.
Sodium tetraphenylborate class toughener can be applicable to horseradish peroxidase enzyme catalytic luminol,3-aminophthalic acid cyclic hydrazide-hydrogen peroxide chemiluminescence reaction system.Use sodium tetraphenylborate to design the test kit that is used for immunochemiluminometry as toughener, comprising luminol,3-aminophthalic acid cyclic hydrazide, hydrogen peroxide, sodium tetraphenylborate is coated with the enzyme-linked reaction plate of antibody, standard antigen, enzyme labelled antibody or enzyme mark streptavidin, biotinylated antibody etc.
The discovery of this new toughener can cause a class to have the development and application of the toughener of similar structures.Along with the use of this class toughener, for the mensuration of horseradish peroxidase and the chemiluminescence enzyme immunoassay of enzyme labelling thereof provide new mensuration system.This toughener is soluble in water, is different from organic substances such as phenols and need be dissolved in organic solvent, and this has special advantage in mensuration, preservation and kit developing.
Embodiment provided by the invention is as follows:
Embodiment 1: utilize sodium tetraphenylborate to measure thyroxine (T4) as the luminous reaction toughener.
1). wrapper sheet:, make insolubilized antibody with the T4 antibody sandwich micro reaction plate of purifying.
With the carbonate buffer solution of 0.1mol/L pH9.6 with the T4 antibody dilution to 10 μ g/ml, get 100 μ l and add in the micropore, seal back 4 ℃ and spend the night.Inferior daily 0.01mol/L pH7.4 PBS washing three times adds 0.01mol/L pH7.4 PBS, and 37 ℃ of sealing 30min are standby with 0.2mol/L pH8.6 boric acid-borate buffer solution washing 3 times.
2). measure: plate is washed 3 times with washings, got rid of surplus liquid.In control wells, standard orifice and testing sample hole add blank solution respectively, reference liquid and testing sample 50 μ l, marker 100 μ l. fully shake up 37 ℃ 1 hour, wash plate 5 times, dry.Every hole adds freshly prepared luminol,3-aminophthalic acid cyclic hydrazide working fluid 50 μ l, hydrogen peroxide 50 μ l, sodium tetraphenylboron 50 μ l in regular turn.Place immediately and detect luminous intensity on the luminescence analyzer, about 1 second of Measuring Time.Measuring sensitivity is 4.0 μ g/dL.
Embodiment 2: utilize sodium tetraphenylborate to measure Regular Insulin as the luminous reaction toughener.
1). wrapper sheet: the globefish anti-insulin antibody bag of using purifying is made insolubilized antibody by micro reaction plate.
Carbonate buffer solution with 0.1mol/L pH9.6 is diluted to 10 μ g/ml with the globefish anti-insulin antibody, gets 100 μ l and adds in the micropore, seals back 4 ℃ and spends the night.Inferior daily 0.01mol/L pH7.4PBS washing three times adds 0.01mol/L pH7.4PBS, and 37 ℃ of sealing 30min are standby with 0.2mol/LpH8.6 boric acid-borate buffer solution washing 3 times.
2). measure: plate is washed 3 times with washings, got rid of surplus liquid.In control wells, standard orifice and testing sample hole add blank solution respectively, reference liquid and testing sample 50 μ l, marker 100 μ l. fully shake up 37 ℃ 1 hour, wash plate 5 times, dry.Every hole adds freshly prepared luminol,3-aminophthalic acid cyclic hydrazide working fluid 50 μ l, hydrogen peroxide 50 μ l, sodium tetraphenylboron 50 μ l in regular turn.Place immediately and detect luminous intensity on the luminescence analyzer, about 1 second of Measuring Time.Mensuration sensitivity is 0.1ng.
Embodiment 3: utilize sodium tetraphenylborate to measure triiodothyronine (T3) as the luminous reaction toughener
1). wrapper sheet: with the T of purifying 3The antibody sandwich micro reaction plate is made insolubilized antibody.
With the carbonate buffer solution of 0.1mol/L pH9.6 with the T3 antibody dilution to 10 μ g/ml, get 100 μ l and add in the micropore, seal back 4 ℃ and spend the night.Inferior daily 0.01mol/L pH7.4 PBS washing three times adds 0.01mol/L pH7.4 PBS, and 37 ℃ of sealing 30min are standby with 0.2mol/L pH8.6 boric acid-borate buffer solution washing 3 times.
2). measure: plate is washed 3 times with washings, got rid of surplus liquid.In control wells, standard orifice and testing sample hole add blank solution respectively, reference liquid and testing sample 50 μ l, marker 100 μ l. fully shake up 37 ℃ 1 hour, wash plate 5 times, dry.Every hole adds freshly prepared luminol,3-aminophthalic acid cyclic hydrazide working fluid 50 μ l, hydrogen peroxide 50 μ l, sodium tetraphenylboron 50 μ l in regular turn.Place immediately and detect luminous intensity on the luminescence analyzer, about 1 second of Measuring Time.Mensuration sensitivity is 25ng/dL.

Claims (1)

1. the application of a sodium tetraphenylborate, this sodium tetraphenylborate has following structure:
It is characterized in that it can be as the novel enhanced agent of enzyme-catalyzed chemical luminescence reaction.
CN 98125659 1998-12-24 1998-12-24 Intensifier for enzymatically chemical luminous reaction Expired - Fee Related CN1311053C (en)

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Application Number Priority Date Filing Date Title
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Application Number Priority Date Filing Date Title
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CN1311053C true CN1311053C (en) 2007-04-18

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Families Citing this family (6)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN1318538C (en) * 2004-08-30 2007-05-30 北京源德生物医学工程有限公司 Sensitivity-reinforced chemical light-emitting liquid containing auxiliary intensifier and intensifier
CN1924580B (en) * 2005-08-30 2010-04-14 郑州安图绿科生物工程有限公司 Chemical luminescent analysis reagent kid for quantitatively detecting trilute
CN104049080B (en) * 2014-06-27 2016-07-20 中国农业科学院农业质量标准与检测技术研究所 Chemiluminescence enhanced sensitivity liquid and preparation method thereof
CN104897909A (en) * 2015-05-02 2015-09-09 王贤俊 Luteinizing hormone (LH)chemiluminescence immunoassay quantitative determination kit
CN104849475A (en) * 2015-05-02 2015-08-19 王贤俊 Quantified detection method for luteinizing hormone (LH)
WO2018000420A1 (en) * 2016-07-01 2018-01-04 深圳市亚辉龙生物科技股份有限公司 Chemiluminescence enhancer and chemiluminescence immunodetection kit

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