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大肠杆菌素受体的定位与增溶

Localization and solubilization of colicin receptors.

作者信息

Sabet S F, Schnaitman C A

出版信息

J Bacteriol. 1971 Oct;108(1):422-30. doi: 10.1128/jb.108.1.422-430.1971.

Abstract

Envelope fractions isolated from Escherichia coli K-12 C600 and from colicin-resistant and colicin-tolerant (Tol II) mutants derived from this strain were separated on sucrose gradients into cell wall-enriched and cytoplasmic membrane-enriched fractions. These fractions were tested for their ability to neutralize colicins of the E and K groups. Neutralization activity was found in the cell wall-enriched fraction from the parent and the Tol II mutant but was absent from all fractions from the resistant mutant. This was also tested with several other E. coli strains. In all cases, sensitive strains contained the neutralization activity, whereas resistant strains did not. The neutralization activity was solubilized from cell walls or cell envelopes of sensitive or Tol II strains by extraction at room temperature with Triton X-100 plus ethylenediaminetetraacetic acid. The solubilized activity was precipitated by 20% ammonium sulfate, 70% ethanol, or 10% trichloroacetic acid. The activity was destroyed by treatment of the solubilized preparation with trypsin or periodate. These results suggest that this colicin-neutralization activity is due to the presence of specific receptors localized in the cell wall and that intact protein and a carbohydrate are required for this receptor to bind colicin.

摘要

从大肠杆菌K-12 C600以及由此菌株衍生的抗大肠杆菌素和耐大肠杆菌素(Tol II)突变体中分离出的包膜级分,在蔗糖梯度上分离成富含细胞壁的级分和富含细胞质膜的级分。测试了这些级分中和E组和K组大肠杆菌素的能力。在亲本和Tol II突变体的富含细胞壁的级分中发现了中和活性,但在抗性突变体的所有级分中均未发现。还用其他几种大肠杆菌菌株进行了测试。在所有情况下,敏感菌株都具有中和活性,而抗性菌株则没有。通过在室温下用Triton X-100加乙二胺四乙酸从敏感或Tol II菌株的细胞壁或细胞包膜中溶解中和活性。溶解的活性可被20%硫酸铵、70%乙醇或10%三氯乙酸沉淀。用胰蛋白酶或高碘酸盐处理溶解的制剂会破坏活性。这些结果表明,这种大肠杆菌素中和活性是由于细胞壁中存在特定受体,并且该受体结合大肠杆菌素需要完整的蛋白质和碳水化合物。

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Localization and solubilization of colicin receptors.大肠杆菌素受体的定位与增溶
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MECHANISM OF ACTION OF COLICINES.大肠杆菌素的作用机制
Proc Natl Acad Sci U S A. 1964 Dec;52(6):1514-21. doi: 10.1073/pnas.52.6.1514.
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