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肺炎球菌的转化:隐蔽期复合体的蛋白质含量

Transformation in pneumococcus: protein content of eclipse complex.

作者信息

Morrison D A

出版信息

J Bacteriol. 1978 Nov;136(2):548-57. doi: 10.1128/jb.136.2.548-557.1978.

Abstract

A two-step purification of pneumococcal eclipse complex is described, which uses sucrose gradient sedimentation followed by agarose gel permeation chromatography. Purified complex contains, in addition to donor DNA single strands, macromolecular material that can be labeled with methionine or leucine during development of competence. This material co-chromatographed with eclipse complex DNA on hydroxylapatite, was dissociated from the DNA by sodium dodecyl sulfate, and was completely digested by Pronase. The sodium dodecyl sulfate-released material eluted as a single peak in sodium dodecyl sulfate chromatography. These properties were consistent with the noncovalent association with eclipse complex of a protein or class of proteins with a narrow range of polypeptide sizes. Evidence for the specific association of this protein with transforming DNA is eclipse was also obtained from parallel purification from 35S-labeled nontransformed cells; the amount of methionine label in the corresponding fractions in such cells was only 5% of that in transformed cells.

摘要

本文描述了肺炎球菌蚀型复合物的两步纯化方法,该方法先采用蔗糖梯度沉降,然后进行琼脂糖凝胶渗透色谱。纯化后的复合物除了含有供体DNA单链外,还包含在感受态形成过程中可用甲硫氨酸或亮氨酸标记的大分子物质。这种物质在羟基磷灰石上与蚀型复合物DNA共色谱,可被十二烷基硫酸钠从DNA上解离,并被链霉蛋白酶完全消化。十二烷基硫酸钠释放的物质在十二烷基硫酸钠色谱中以单峰形式洗脱。这些特性与一种或一类多肽大小范围较窄的蛋白质与蚀型复合物的非共价结合相一致。从35S标记的未转化细胞进行平行纯化也获得了这种蛋白质与转化DNA特异性结合的证据;此类细胞相应组分中甲硫氨酸标记量仅为转化细胞中的5%。

相似文献

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Localization of competence-induced proteins in Streptococcus pneumoniae.
J Bacteriol. 1986 Mar;165(3):689-95. doi: 10.1128/jb.165.3.689-695.1986.

引用本文的文献

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Localization of competence-induced proteins in Streptococcus pneumoniae.
J Bacteriol. 1986 Mar;165(3):689-95. doi: 10.1128/jb.165.3.689-695.1986.

本文引用的文献

9
Breakage prior to entry of donor DNA in Pneumococcus transformation.肺炎球菌转化过程中供体DNA进入前的断裂
Biochim Biophys Acta. 1973 Apr 11;299(4):545-56. doi: 10.1016/0005-2787(73)90226-8.

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