Recombinant Gaussia luciferase with a reactive cysteine residue for chemical conjugation: expression, purification and its application for bioluminescent immunoassays.

Inouye S; Sato J; Sahara Miura Y

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Recombinant Gaussia luciferase with a reactive cysteine residue for chemical conjugation: expression, purification and its application for bioluminescent immunoassays.

机译：带有活性半胱氨酸残基的重组高斯荧光素酶用于化学偶联：表达，纯化及其在生物发光免疫分析中的应用。

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The mutated recombinant Gaussia luciferase (hgGLase) having the hinge sequence with a reactive cysteine residue at the carboxyl terminal region was purified from Escherichia coli cells by nickel-chelate affinity chromatography and hydrophobic chromatography. The biotinylated hgGLase (Biotin-hgGLase) was prepared by chemical conjugation with a maleimide activated biotin and apply to bioluminescent immunoassay. In the streptavidin and biotin complex system using Biotin-hgGLase, the measurable range of alpha-fetoprotein as a model analyte was 0.02-100ng/ml with the coefficient of variation between 2.5% and 5.2%. The sensitivity of Biotin-hgGLase was similar to that by using the detection system of aequorin, alkaline phosophatase and horseradish peroxidase as a label enzyme.

机译：通过镍螯合亲和层析和疏水层析从大肠杆菌细胞中纯化了具有在羧基末端区域具有反应性半胱氨酸残基的铰链序列的突变的重组高斯荧光素酶（hgGLase）。通过与马来酰亚胺活化的生物素化学缀合来制备生物素化的hgGLase（Biotin-hgGLase），并将其应用于生物发光免疫测定。在使用生物素-hgGLase的链霉亲和素和生物素复合物系统中，作为模型分析物的甲胎蛋白的可测量范围为0.02-100ng / ml，变异系数在2.5％和5.2％之间。通过使用水母发光蛋白，碱性磷酸酶和辣根过氧化物酶的检测系统作为标记酶，生物素-hgGLase的敏感性与之相似。

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《Biochemical and Biophysical Research Communications》 |2011年第4期|共6页
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Inouye S; Sato J; Sahara Miura Y;
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2. Recombinant Gaussia luciferase with a reactive cysteine residue for chemical conjugation: expression, purification and its application for bioluminescent immunoassays. [J] . Inouye S, Sato J, Sahara Miura Y Biochemical and Biophysical Research Communications . 2011,第4期

机译：带有活性半胱氨酸残基的重组高斯荧光素酶用于化学偶联：表达，纯化及其在生物发光免疫分析中的应用。
3. Recombinant Gaussia luciferase. Overexpression, purification, and analytical application of a bioluminescent reporter for DNA hybridization [J] . Verhaegen M., Christopoulos TK. Analytical chemistry . 2002,第17期

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4. Purification of histidine-tagged aequorin with a reactive cysteine residue for chemical conjugations and its application for bioluminescent sandwich immunoassays [J] . Satoshi Inouye, Jun-ichi Sato Protein Expression and Purification . 2012,第2期

机译：具有反应性半胱氨酸残基的组氨酸标记的水母发光蛋白的纯化，用于化学缀合及其在生物发光夹心免疫分析中的应用
5. NOVEL BRET-BASED BIOSENSORS WITH A NEW BIOLUMINESCENT DONOR, GAUSSIA LUCIFERASE, FOR ESTROGEN RECEPTOR LIGANDS [C] . E MICHELINI, M MAGLIULO, M BARALDINI, International Symposium on Bioluminescence and Chemiluminescence . 2007

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6. Engineering, overexpression, purification and analytical applications of recombinant bioluminescent reporters [D] . Verhaegen, Monique Elise 2002

机译：重组生物发光报告基因的工程，过表达，纯化和分析应用
7. Gaussia princeps luciferase: a bioluminescent substrate for oxidative protein folding [O] . Tiantian Yu, Joanna R. Laird, Jennifer A. Prescher, 2018

机译：Gaussia princeps荧光素酶：氧化蛋白折叠的生物发光底物
8. Engineering, overexpression, purification and analytical applications of recombinant bioluminescent reporters. [O] . Verhaegen Monique Elise. 2002

机译：重组生物发光报告基因的工程，过表达，纯化和分析应用。

Recombinant Gaussia luciferase with a reactive cysteine residue for chemical conjugation: expression, purification and its application for bioluminescent immunoassays.

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