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慢生根瘤菌中镍的积累与储存

Nickel accumulation and storage in Bradyrhizobium japonicum.

作者信息

Maier R J, Pihl T D, Stults L, Sray W

机构信息

Department of Biology, Johns Hopkins University, Baltimore, Maryland 21218.

出版信息

Appl Environ Microbiol. 1990 Jun;56(6):1905-11. doi: 10.1128/aem.56.6.1905-1911.1990.

DOI:10.1128/aem.56.6.1905-1911.1990
PMID:2200341
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC184529/
Abstract

Hydrogenase-derepressed (chemolithotrophic growth conditions) and heterotrophically grown cultures of Bradyrhizobium japonicum accumulated nickel about equally over a 3-h period. Both types of cultures accumulated nickel primarily in a form that was not exchangeable with NiCl2, and they accumulated much more Ni than would be needed for the Ni-containing hydrogenase. The nickel accumulated by heterotrophically incubated cultures could later be mobilized to allow active hydrogenase synthesis during derepression in the absence of nickel, while cells both grown and derepressed without nickel had low hydrogenase activities. The level of activity in cells grown with Ni and then derepressed without nickel was about the same as that in cultures derepressed in the presence of nickel. The Ni accumulated by heterotrophically grown cultures was associated principally with soluble proteins rather than particulate material, and this Ni was not lost upon dialyzing an extract containing the soluble proteins against either Ni-containing or EDTA-containing buffer. However, this Ni was lost upon pronase or low pH treatments. The soluble Ni-binding proteins were partially purified by gel filtration and DEAE chromatography. They were not antigenically related to hydrogenase peptides. Much of the 63Ni eluted as a single peak of 48 kilodaltons. Experiments involving immunoprecipitation of 63Ni-containing hydrogenase suggested that the stored source of Ni in heterotrophic cultures that could later be mobilized into hydrogenase resided in the nonexchangeable Ni-containing fraction rather than in loosely bound or ionic forms.

摘要

在3小时的时间段内,氢化酶去阻遏(化学无机营养生长条件)的日本慢生根瘤菌培养物和异养生长的培养物积累的镍量大致相同。这两种类型的培养物积累的镍主要以一种不能与氯化镍交换的形式存在,并且它们积累的镍比含镍氢化酶所需的镍多得多。异养培养的培养物积累的镍后来可以被动员起来,以便在无镍的去阻遏过程中进行活跃的氢化酶合成,而在无镍条件下生长和去阻遏的细胞氢化酶活性较低。在有镍的情况下生长然后在无镍条件下去阻遏的细胞中的活性水平与在有镍存在下去阻遏的培养物中的活性水平大致相同。异养生长的培养物积累的镍主要与可溶性蛋白质相关,而不是与颗粒物质相关,并且当用含镍或含乙二胺四乙酸(EDTA)的缓冲液透析含有可溶性蛋白质的提取物时,这种镍不会丢失。然而,在用链霉蛋白酶或低pH处理后,这种镍会丢失。通过凝胶过滤和二乙氨基乙基(DEAE)色谱法对可溶性镍结合蛋白进行了部分纯化。它们与氢化酶肽没有抗原相关性。大部分63Ni以一个48千道尔顿的单峰形式洗脱。涉及对含63Ni氢化酶进行免疫沉淀的实验表明,异养培养物中可储存的镍源,即后来可被动员到氢化酶中的镍源,存在于不可交换的含镍部分,而不是以松散结合或离子形式存在。

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