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J. Bacteriol., Jul 1995, 3704-3713, Vol 177, No. 13
J Cao, AS Khan, ME Bayer and DM Schifferli
The 987P fimbria of enterotoxigenic Escherichia coli is a heteropolymeric
structure which consists essentially of a major FasA subunit and a minor
subunit, the FasG adhesin. The latter harbors the binding moiety for
receptor molecules on piglet intestinal epithelial cells. In this study,
anti-FasF antibody probes were developed and used to demonstrate that the
FasF protein represents a new minor fimbrial component. FasF was identified
in highly purified fimbriae, and its sequence demonstrated significant
levels of similarity with that of FasA. Immune electron microscopy
localized both the FasG and FasF proteins at the fimbrial tip as well as at
broken ends and at various intervals along the fimbrial length. The
presence of these minor proteins in purified 987P fimbriae was corroborated
by enzyme-linked immunosorbent assay inhibitions. Finally, the use of
nonfimbriated fasG, fasF, and fasA mutants indicated that subunit
translocation through the outer membrane follows a specific order, FasG
being the first, FasF being the second, and FasA being the third type of
exported subunit. Since fimbriae are thought to grow from the base, FasG is
proposed to be a tip adhesin and FasF is proposed to be a linker molecule
between the adhesin and the fimbrial shaft. Moreover, export of FasG (or
FasF) in the absence of FasF (or FasA) indicates that during the process of
fimbrial biogenesis in the outer membrane, translocating events precede the
initiation of subunit heteropolymerization.
Copyright © 1995, American Society for Microbiology
Ordered translocation of 987P fimbrial subunits through the outer membrane of Escherichia coli
Department of Pathobiology, University of Pennsylvania School of Veterinary Medicine, Philadelphia 19104, USA.
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