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镁及MgtC在鼠伤寒沙门氏菌生长中的作用。

Magnesium and the role of MgtC in growth of Salmonella typhimurium.

作者信息

Moncrief M B, Maguire M E

机构信息

Department of Pharmacology, School of Medicine, Case Western Reserve University, Cleveland, Ohio 44106-4965, USA.

出版信息

Infect Immun. 1998 Aug;66(8):3802-9. doi: 10.1128/IAI.66.8.3802-3809.1998.

Abstract

Salmonella typhimurium has three distinct transport systems for Mg2+: CorA, MgtA, and MgtB. The mgtCB operon encodes two proteins, MgtC, a hydrophobic protein with a predicted molecular mass of 22.5 kDa, and MgtB, a 102-kDa P-type ATPase Mg2+ transport protein. The mgtCB locus has been identified as part of a new Salmonella pathogenicity island, SPI-3. Transcription of mgtCB is regulated by extracellular Mg2+ via the two-component PhoPQ regulatory system important for virulence. To elucidate MgtC's role in a low-Mg2+ environment, we looked at growth and transport in strains lacking the CorA and MgtA Mg2+ transporters but expressing MgtB, MgtC, or both. mgtC mgtB+ and mgtC+ mgtB+ strains exhibited growth in N minimal medium without added Mg2+ with a 1- to 2-h lag phase. An mgtC+ mgtB strain was also able to grow in N minimal medium without added Mg2+ but only after a 24-h lag phase. In N minimal medium containing 10 mM Mg2+, all strains grew after a short lag phase; the mgtC+ mgtB strain grew to a higher optical density at 600 nm than an mgtC+ mgtB+ strain and was comparable to wild type. The lengthy lag phase before growth in an mgtC+ mgtB strain was not due to lack of expression of MgtC. Western blot analysis indicated that substantial MgtC protein is present by 2 h after suspension in N minimal medium. Surprisingly, in an mgtC+ mgtB+ strain, MgtC was undetectable during Mg2+ starvation, although large amounts of MgtB were observed. The lack of expression of MgtC is not dependent on functional MgtB, since a strain carrying a nonfunctional MgtB with a mutation (D379A) also did not make MgtC. Since, during invasion of eukaryotic cells, S. typhimurium appears to be exposed to a low-pH as well as a low-Mg2+ environment, the growth of an mgtC+ mgtB strain was tested at low pH with and without added Mg2+. While significant quantities of MgtC could be detected after suspension at pH 5.2, the mgtC+ mgtB strain was unable to grow at pH 5.2 whether or not Mg2+ was present. Finally, using 63Ni2+ and 57Co2+ as alternative substrates for the unavailable 28Mg2+, cation uptake could not be detected in an mgtC+ mgtB strain after Mg2+ starvation. We conclude that MgtC is not a Mg2+ transporter and that it does not have a primary role in the survival of S. typhimurium at low pH.

摘要

鼠伤寒沙门氏菌有三种不同的镁离子(Mg2+)转运系统:CorA、MgtA和MgtB。mgtCB操纵子编码两种蛋白质,MgtC,一种预测分子量为22.5 kDa的疏水蛋白,以及MgtB,一种102 kDa的P型ATP酶镁离子转运蛋白。mgtCB基因座已被鉴定为新的沙门氏菌致病岛SPI-3的一部分。mgtCB的转录受细胞外镁离子通过对毒力很重要的双组分PhoPQ调节系统调控。为了阐明MgtC在低镁离子环境中的作用,我们研究了缺乏CorA和MgtA镁离子转运蛋白但表达MgtB、MgtC或两者的菌株的生长和转运情况。mgtC mgtB+和mgtC+ mgtB+菌株在不添加镁离子的N基本培养基中表现出生长,有1至2小时的延迟期。mgtC+ mgtB菌株也能够在不添加镁离子的N基本培养基中生长,但仅在24小时的延迟期后。在含有10 mM镁离子的N基本培养基中,所有菌株在短暂的延迟期后都生长;mgtC+ mgtB菌株在600 nm处的光密度比mgtC+ mgtB+菌株更高,且与野生型相当。mgtC+ mgtB菌株生长前的长时间延迟期不是由于MgtC表达不足。蛋白质印迹分析表明,在悬浮于N基本培养基中2小时后,大量的MgtC蛋白存在。令人惊讶的是,在mgtC+ mgtB+菌株中,在镁离子饥饿期间未检测到MgtC,尽管观察到大量的MgtB。MgtC的缺乏表达不依赖于功能性的MgtB,因为携带无功能MgtB(D379A突变)的菌株也不产生MgtC。由于在入侵真核细胞期间,鼠伤寒沙门氏菌似乎暴露于低pH以及低镁离子环境中,因此测试了mgtC+ mgtB菌株在添加和不添加镁离子的低pH条件下的生长情况。虽然在pH 5.2悬浮后可以检测到大量的MgtC,但无论是否存在镁离子,mgtC+ mgtB菌株在pH 5.2时都无法生长。最后,使用63Ni2+和57Co2+作为不可用的28Mg2+的替代底物,在镁离子饥饿后的mgtC+ mgtB菌株中未检测到阳离子摄取。我们得出结论,MgtC不是镁离子转运蛋白,并且它在鼠伤寒沙门氏菌在低pH下的存活中没有主要作用。

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