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NADH氧化酶光镜检测中的陷阱

Pitfalls in the light microscopical detection of NADH oxidase.

作者信息

Gossrau R, Van Noorden C J, Frederiks W M

机构信息

Department of Anatomy, Free University of Berlin, Germany.

出版信息

Histochem J. 1990 Mar;22(3):155-61. doi: 10.1007/BF01003535.

Abstract

NADH oxidase activity has been detected at the ultrastructural level using cerium ions to trap H2O2 generated by the enzyme (via intermediate reactive oxygen species). In an attempt to localize NADH oxidase activity at the light microscope level using the cerium-diaminobenzidine (DAB)-nickel-H2O2, the cerium-DAB-cobalt-H2O2 or the cerium-alkaline lead procedures, the distribution patterns of the revealed enzyme were found to be identical to those for non-specific alkaline phosphatase and especially 5'-nucleotidase activity. With the cerium-DAB-cobalt-H2O2 visualization procedure, the distribution pattern of the final reaction product was similar to that obtained with the other two techniques but much less final reaction product was formed. Incubations for NADH oxidase activity performed in the presence of exogenous catalase or in the absence of catalase or peroxidase inhibitors did not affect the staining intensity, whereas inhibitors of 5'-nucleotidase (EDTA) and non-specific alkaline phosphatase (levamisole) always did. Therefore, phosphatases contribute to the formation of the final reaction product. Since NADH initially cannot be hydrolysed by either of these two phosphatases, then presumably nucleotide pyrophosphatase (E.C.3.6.1.9) cleaves NADH into 5'-AMP and nicotinamide mononucleotide in a first step. Both nucleotides can be hydrolysed further by the two monophosphatases. These then generate cerium phosphate which is detected by the DAB-nickel-H2O2, DAB-cobalt-H2O2 or lead visualization methods.

摘要

利用铈离子捕获该酶产生的H2O2(通过中间活性氧物种),已在超微结构水平检测到NADH氧化酶活性。为了在光学显微镜水平使用铈 - 二氨基联苯胺(DAB) - 镍 - H2O2、铈 - DAB - 钴 - H2O2或铈 - 碱性铅法定位NADH氧化酶活性,发现所揭示的酶的分布模式与非特异性碱性磷酸酶尤其是5'-核苷酸酶活性的分布模式相同。使用铈 - DAB - 钴 - H2O2可视化程序时,最终反应产物的分布模式与其他两种技术获得的相似,但形成的最终反应产物要少得多。在存在外源性过氧化氢酶的情况下或在不存在过氧化氢酶或过氧化物酶抑制剂的情况下进行的NADH氧化酶活性孵育不影响染色强度,而5'-核苷酸酶(EDTA)和非特异性碱性磷酸酶(左旋咪唑)的抑制剂总是会影响。因此,磷酸酶有助于最终反应产物的形成。由于NADH最初不能被这两种磷酸酶中的任何一种水解,那么推测核苷酸焦磷酸酶(E.C.3.6.1.9)在第一步中将NADH裂解为5'-AMP和烟酰胺单核苷酸。这两种核苷酸都可以被两种单磷酸酶进一步水解。然后它们产生磷酸铈,通过DAB - 镍 - H2O2、DAB - 钴 - H2O2或铅可视化方法检测。

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