Additional In Vitro and In Vivo Evidence for SecA Functioning as Dimers in the Membrane: Dissociation into Monomers Is Not Essential for Protein Translocation in
            <i>Escherichia coli</i>

Wang, Hongyun; Na, Bing; Yang, Hanfang; Tai, Phang C.

doi:10.1128/jb.01633-07

Cited by 37 publications

(57 citation statements)

References 33 publications

(51 reference statements)

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“…At 100 mM KCl, the SecA (no His) dimer is only approximately 10-fold tighter than that of SecA ⌬2-11 (Table 1). This finding is consistent with previous studies, in which SecA ⌬2-11/N95 was found to exist primarily in the dimeric state in low-ionic-strength buffers (43,44).…”

Section: Resultssupporting

confidence: 83%

“…In addition, SecA F263X and F10X produce a cross-linked dimer band with a faster electrophoretic mobility than other variants. The aberrant SDS-PAGE mobilities may result from changes in conformation dependent on the location of cross-linked residues (34), as observed in previous chemical cross-linking experiments (17,28,44).…”

Section: Resultsmentioning

confidence: 83%

“…Moreover, formaldehyde cross-linking, which links amino acids in very close proximity, also showed dimeric SecA ⌬2-11/N95 in vivo (44). This suggests that experiments such as those evaluating specific cysteine-cysteine cross-linking that indicate that SecA ⌬2-11/N95 is monomeric must be interpreted cautiously (17).…”

Section: Figmentioning

confidence: 99%

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Defining the Escherichia coli SecA Dimer Interface Residues through In Vivo Site-Specific Photo-Cross-Linking

Wowor

Cole

et al. 2013

J Bacteriol

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The motor protein SecA is a core component of the bacterial general secretory (Sec) pathway and is essential for cell viability. Despite evidence showing that SecA exists in a dynamic monomer-dimer equilibrium favoring the dimeric form in solution and in the cytoplasm, there is considerable debate as to the quaternary structural organization of the SecA dimer. Here, a site-directed photo-cross-linking technique was utilized to identify residues on the Escherichia coli SecA (ecSecA) dimer interface in the cytosol of intact cells. The feasibility of this method was demonstrated with residue Leu6, which is essential for ecSecA dimerization based on our analytical ultracentrifugation studies of SecA L6A and shown to form the cross-linked SecA dimer in vivo with p-benzoyl-phenylalanine (pBpa) substituted at position 6. Subsequently, the amino terminus (residues 2 to 11) in the nucleotide binding domain (NBD), Phe263 in the preprotein binding domain (PBD), and Tyr794 and Arg805 in the intramolecular regulator of the ATPase 1 domain (IRA1) were identified to be involved in ecSecA dimerization. Furthermore, the incorporation of pBpa at position 805 did not form a cross-linked dimer in the SecA ⌬2-11 context, indicating the possibility that the amino terminus may directly contact Arg805 or that the deletion of residues 2 to 11 alters the topology of the naturally occurring ecSecA dimer.

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Section: Resultssupporting

confidence: 83%

Section: Resultsmentioning

confidence: 83%

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Defining the Escherichia coli SecA Dimer Interface Residues through In Vivo Site-Specific Photo-Cross-Linking

Wowor

Cole

et al. 2013

J Bacteriol

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“…However, a recent single-molecule study suggested that the dimeric organization of SecA is maintained when actively engaged in preprotein translocation [93]. Covalent stabilization of the SecA dimer by crosslinking did not interfere with the protein translocation activity [93,103,108,109]. In this respect, the T. maritima SecYEG-SecA crystal structure shows a monomer of SecA bound to SecYEG, but this structure may not reflect the physiological oligomeric state of SecA as the crystallization process was accompanied with detergents and high salt, both of which have been shown to negate interactions in a SecA dimer interface [93,106].…”

Section: The Motor Protein Secamentioning

confidence: 99%

The bacterial Sec-translocase: structure and mechanism

Nijeholt

Driessen

2012

Phil. Trans. R. Soc. B

147

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Most bacterial secretory proteins pass across the cytoplasmic membrane via the translocase, which consists of a protein-conducting channel SecYEG and an ATP-dependent motor protein SecA. The ancillary SecDF membrane protein complex promotes the final stages of translocation. Recent years have seen a major advance in our understanding of the structural and biochemical basis of protein translocation, and this has led to a detailed model of the translocation mechanism.

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“…Both in vivo and in vitro protein cross-linking techniques have been utilized to assess the fraction of the SecA dimer in soluble and membrane-bound states. Unfortunately, the studies have produced equivocal results (17,23,24,32) that are of limited value; on the one hand, cross-linking traps proteins in the oligomeric state and thus distorts a natural equilibrium, while on the other hand, suboptimal cross-linking conditions (e.g., nonideal cross-linker chemistry, insufficient cross-linker concentration, or nonphysiological buffer or salt conditions) can lead to underrepresentation of the true oligomeric population. Genetic techniques have been utilized to engineer SecA dimers that were linked in a head-to-tail fashion, and such modified proteins were found to be functional both in vivo and in vitro (22,32).…”

mentioning

confidence: 99%

Reexamination of the Role of the Amino Terminus of SecA in Promoting Its Dimerization and Functional State

et al. 2008

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The SecA nanomotor promotes protein translocation in eubacteria by binding both protein cargo and the protein-conducting channel and by undergoing ATP-driven conformation cycles that drive this process. There are conflicting reports about whether SecA functions as a monomer or dimer during this dynamic process. Here we reexamined the roles of the amino and carboxyl termini of SecA in promoting its dimerization and functional state by examining three secA mutants and the corresponding proteins: SecA⌬8 lacking residues 2 to 8, SecA⌬11 lacking residues 2 to 11, and SecA⌬11/N95 lacking both residues 2 to 11 and the carboxylterminal 70 residues. We demonstrated that whether SecA⌬11 or SecA⌬11/N95 was functional for promoting cell growth depended solely on the vivo level of the protein, which appeared to govern residual dimerization. All three SecA mutant proteins were defective for promoting cell growth unless they were highly overproduced. Cell fractionation revealed that SecA⌬11 and SecA⌬11/N95 were proficient in membrane association, although the formation of integral membrane SecA was reduced. The presence of a modestly higher level of SecA⌬11/N95 in the membrane and the ability of this protein to form dimers, as detected by chemical cross-linking, were consistent with the higher level of secA expression and better growth of the SecA⌬11/N95 mutant than of the SecA⌬11 mutant. Biochemical studies showed that SecA⌬11 and SecA⌬11/N95 had identical dimerization defects, while SecA⌬8 was intermediate between these proteins and wild-type SecA in terms of dimer formation. Furthermore, both SecA⌬11 and SecA⌬11/N95 were equally defective in translocation ATPase specific activity. Our studies showed that the nonessential carboxyl-terminal 70 residues of SecA play no role in its dimerization, while increasing the truncation of the amino-terminal region of SecA from 8 to 11 residues results in increased defects in SecA dimerization and poor in vivo function unless the protein is highly overexpressed.

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Additional In Vitro and In Vivo Evidence for SecA Functioning as Dimers in the Membrane: Dissociation into Monomers Is Not Essential for Protein Translocation in Escherichia coli

Cited by 37 publications

References 33 publications

Defining the Escherichia coli SecA Dimer Interface Residues through In Vivo Site-Specific Photo-Cross-Linking

Defining the Escherichia coli SecA Dimer Interface Residues through In Vivo Site-Specific Photo-Cross-Linking

The bacterial Sec-translocase: structure and mechanism

Reexamination of the Role of the Amino Terminus of SecA in Promoting Its Dimerization and Functional State

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