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荧光铁载体介导的铜绿假单胞菌 M114 菌株铁摄取的特性:存在额外的三价铁载体受体的证据。

Characterization of Fluorescent Siderophore-Mediated Iron Uptake in Pseudomonas sp. Strain M114: Evidence for the Existence of an Additional Ferric Siderophore Receptor.

机构信息

Microbiology Department, University College, Cork, Ireland, and Department of Molecular Cell Biology, University of Utrecht, Padualaan 8, 3584 CH Utrecht, The Netherlands.

出版信息

Appl Environ Microbiol. 1992 Feb;58(2):630-5. doi: 10.1128/aem.58.2.630-635.1992.

Abstract

In Pseudomonas sp. strain M114, the outer membrane receptor for ferric pseudobactin M114 was shown to transport ferric pseudobactins B10 and A225, in addition to its own. The gene encoding this receptor, which was previously cloned on pCUP3, was localized by Tn5 mutagenesis to a region comprising >1.6 kb of M114 DNA. A mutant (strain M114R1) lacking this receptor was then created by a marker exchange technique. Characterization of this mutant by using purified pseudobactin M114 in radiolabeled ferric iron uptake studies confirmed that it was completely unable to utilize this siderophore for acquisition of iron. In addition, it lacked an outer membrane protein band of 89 kDa when subjected to sodium dodecyl sulfate-polyacrylamide gel electrophoresis. As a result, growth of the mutant was severely restricted under low-iron conditions. However, this phenotype was reversed in the presence of another fluorescent siderophore (pseudobactin MT3A) from Pseudomonas sp. strain MT3A, suggesting the presence of a second receptor in strain M114. Furthermore, wild-type Pseudomonas sp. strain B24 was not able to utilize ferric pseudobactin MT3A, and this phenotype was not reversed upon expression of the M114 receptor encoded on pCUP3. However, a cosmid clone (pMS1047) that enabled strain B24 to utilize ferric pseudobactin MT3A was isolated from an M114 gene bank. Radiolabel transport assays with purified pseudobactin MT3A confirmed this event. Plasmid pMS1047 was shown to encode an outer membrane protein of 81 kDa in strain B24 under iron-limiting conditions; this protein corresponds to a similar protein in strain M114.

摘要

在 Pseudomonas sp. strain M114 中,铁假菌素 M114 的外膜受体被证明除了自身外还能转运铁假菌素 B10 和 A225。这个受体的基因以前是在 pCUP3 上克隆的,通过 Tn5 诱变定位到一个包含 >1.6 kb M114 DNA 的区域。然后通过标记交换技术创建了一个缺乏这种受体的突变体(菌株 M114R1)。使用纯化的假菌素 M114 在放射性标记的铁摄取研究中对该突变体进行特征描述,证实它完全无法利用这种铁载体获取铁。此外,当进行十二烷基硫酸钠-聚丙烯酰胺凝胶电泳时,它缺乏一个 89 kDa 的外膜蛋白带。因此,在低铁条件下,突变体的生长受到严重限制。然而,在另一种来自 Pseudomonas sp. strain MT3A 的荧光铁载体(假菌素 MT3A)存在的情况下,这种表型得到了逆转,这表明菌株 M114 中存在第二种受体。此外,野生型 Pseudomonas sp. strain B24 无法利用铁假菌素 MT3A,并且在表达 pCUP3 上编码的 M114 受体时,这种表型没有得到逆转。然而,从 M114 基因库中分离到一个能够使菌株 B24 利用铁假菌素 MT3A 的 cosmid 克隆(pMS1047)。用纯化的假菌素 MT3A 进行放射性转运试验证实了这一事件。在铁限制条件下,质粒 pMS1047 显示在菌株 B24 中编码一种 81 kDa 的外膜蛋白;这种蛋白与菌株 M114 中的类似蛋白相对应。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1551/195294/c4f6b60fc933/aem00043-0208-a.jpg

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