Infect Immun, May 1998, p. 1928-1933, Vol. 66, No. 5
0019-9567/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Department of Bacteriology and Immunology,
Received 14 August 1997/Returned for modification 21 October
1997/Accepted 15 February 1998
Protectin (CD59) is a glycophosphoinsitol (GPI)-anchored defender
of human cells against lysis by the membrane attack complex of
complement. In this study, we examined whether protectin released from
human cell membranes can incorporate into the surface of gram-negative
bacteria. Analysis by using radiolabeled protectin, immunofluorescence, flow cytometry, and whole-cell enzyme-linked immunosorbent assay demonstrated that protectin bound to
nonencapsulated Escherichia coli EH237 (Re) and EH234 (Ra)
in a calcium-dependent manner. The incorporation required the
GPI-phospholipid moiety since no binding of a phospholipid-free
soluble form of protectin was observed. Mg2+ did not
enhance the binding, and a polysialic acid capsule prevented it (strain IH3080 [O18:K1:H8]). Bound protectin inhibited the C5b-9
neoantigen expression on complement-treated bacteria.
Protection against complement lysis was observed in both a colony
counting assay and a bioluminescence assay, where
viable EH234 bacteria expressing the luciferase gene emitted green
light in the presence of the luciferine substrate. In
general, two- to four-times-higher serum concentrations were
needed to obtain 50% lysis of protectin-coated versus noncoated bacteria. The results indicate that protectin can
incorporate in a functionally active form into the cell
membranes of the two nonencapsulated deep rough E. coli strains studied.
*
Corresponding author. Mailing address: Department of
Bacteriology and Immunology, Haartman Institute, P.O. Box 21 (Haartmaninkatu 3), FIN-00014 University of Helsinki, Helsinki,
Finland. Phone: 358-9-1912 6377. Fax: 358-9-1912 6382. E-mail:
meri{at}helsinki.fi.
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