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氯霉素酶法测定的改进

Improved enzymatic assay of chloramphenicol.

作者信息

Smith A L, Smith D H

出版信息

Clin Chem. 1978 Sep;24(9):1452-7.

PMID:99271
Abstract

We partly purified R-factor-encoded chloramphenicol acetyltransferase (EC 2.3.1.28) from a highly choloramphenicol-resistant mutant derived from Escherichia coli W677/R5. The preparation permitted rapid quanitation of chloramphenicol by use of [14C]acetylcoenzyme A, removing the diacetylated product by selective adsorption onto micropore filters. Succinyl and glucuronyl 3-hydroxyl esters of chloramphenicol were not active as substrates for the preparation, nor were they active as inhibitors. The enzyme was free of chloramphenicol reductase activity, and utilizes other biologically active chloramphenicol analogs. Other antibiotics, at concentrations commonly found in human sera, and blood preservatives, at concentrations 10-fold that found in blood-collection tubes, did not interfere with the enzymic quantitation of chloramphenicol. We conclude that this enzyme preparation permits rapid clinical quantitation of chloramphenicol.

摘要

我们从源自大肠杆菌W677/R5的高耐氯霉素突变体中部分纯化了R因子编码的氯霉素乙酰转移酶(EC 2.3.1.28)。该制剂允许使用[14C]乙酰辅酶A快速定量氯霉素,通过选择性吸附到微孔滤膜上去除二乙酰化产物。氯霉素的琥珀酰酯和葡糖醛酸3 - 羟基酯不作为该制剂的底物,也不作为抑制剂。该酶没有氯霉素还原酶活性,并且能利用其他具有生物活性的氯霉素类似物。在人血清中常见浓度的其他抗生素以及在采血试管中浓度为10倍的血液防腐剂,均不干扰氯霉素的酶定量测定。我们得出结论,这种酶制剂允许对氯霉素进行快速临床定量。

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