鼠伤寒沙门氏菌鞭毛基体外膜L环脂蛋白FlgH的生理生化分析
Physiological and biochemical analyses of FlgH, a lipoprotein forming the outer membrane L ring of the flagellar basal body of Salmonella typhimurium.
作者信息
Schoenhals G J, Macnab R M
机构信息
Department of Molecular Biophysics and Biochemistry, Yale University, New Haven, Connecticut 06520-8114, USA.
出版信息
J Bacteriol. 1996 Jul;178(14):4200-7. doi: 10.1128/jb.178.14.4200-4207.1996.
The FlgH protein of Salmonella typhimurium, from which the outer membrane L ring of the flagellar basal body is constructed, has a consensus motif (LTG C) for lipoylation and signal peptide cleavage. We have confirmed the previous finding (M. Homma, K. Ohnishi, T. Iino, and R. M. Macnab, J. Bacteriol. 169:3617-3624, 1987) that it is synthesized in precursor form and processed to a mature form with an apparent molecular mass of ca. 25 kDa. flgH alleles with an in-frame deletion or a 3' truncation still permitted processing. The deletion permitted partial restoration of motility in complementation tests, whereas the truncation did not. Globomycin, an antibiotic which inhibits signal peptide cleavage of prolipoproteins, caused accumulation of precursor forms of FlgH. When cells transformed with a plasmid containing the flgH gene were grown in the presence of [3H]palmitate, a 25-kDa protein doublet was found to be radiolabeled; its identity as FlgH was confirmed by shifts in mobility when the internally deleted and truncated alleles of the gene were used. Hook-basal body complexes from cells grown in the presence of [3H]palmitate demonstrated that FlgH incorporated into flagellar structure was also labeled. An in-frame fusion between the leader sequence of the periplasmic protein PeIB and the mature FlgH sequence, with the putative N-terminal cysteine replaced by glycine, resulted in production of a fusion protein that was processed to its mature form. With a low-copy-number plasmid, the ability of this pelB-flgH fusion to complement a flgH mutant was poor, but with a high-copy-number plasmid, it was comparable to that of the wild type. Although lacking the N-terminal cysteine and therefore being incapable of lipoylation via a thioether linkage, the mutant protein still incorporated [3H]palmitate at low levels, perhaps through acylation of the N-terminal alpha-amino group. We conclude that FlgH is a lipoprotein and that under normal physiological conditions the lipoyl modification is necessary for FlgH to function properly as the L-ring protein of the flagellar basal body. We suggest that the N terminus of FlgH is responsible for anchoring the basal body in the outer membrane and that the C terminus may be responsible for binding to the P ring to form the L,P-ring complex.
鼠伤寒沙门氏菌的FlgH蛋白构成鞭毛基体的外膜L环,具有用于硫辛酸化和信号肽切割的共有基序(LTG C)。我们证实了之前的发现(M. 本间、大西健、饭野哲和R. M. 麦克纳布,《细菌学杂志》169:3617 - 3624,1987年),即它以前体形式合成,并加工成表观分子量约为25 kDa的成熟形式。具有框内缺失或3'端截短的flgH等位基因仍允许加工。在互补试验中,缺失允许部分恢复运动性,而截短则不能。球蛋白霉素是一种抑制前脂蛋白信号肽切割的抗生素,导致FlgH前体形式的积累。当用含有flgH基因的质粒转化的细胞在[3H]棕榈酸存在下生长时,发现一个25 kDa的蛋白双峰被放射性标记;当使用该基因的内部缺失和截短等位基因时,其迁移率的变化证实了它就是FlgH。在[3H]棕榈酸存在下生长的细胞的钩 - 基体复合物表明,整合到鞭毛结构中的FlgH也被标记。周质蛋白PeIB的前导序列与成熟的FlgH序列之间的框内融合,将推定的N端半胱氨酸替换为甘氨酸,导致产生一种加工成成熟形式的融合蛋白。使用低拷贝数质粒时,这种pelB - flgH融合体互补flgH突变体的能力较差,但使用高拷贝数质粒时,其能力与野生型相当。尽管缺乏N端半胱氨酸,因此无法通过硫醚键进行硫辛酸化,但突变蛋白仍能以低水平掺入[3H]棕榈酸,可能是通过N端α - 氨基的酰化。我们得出结论,FlgH是一种脂蛋白,在正常生理条件下,硫辛酸修饰对于FlgH作为鞭毛基体的L环蛋白正常发挥功能是必需的。我们认为FlgH的N端负责将基体锚定在外膜中,而C端可能负责与P环结合形成L、P环复合物。
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