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The deletion of 70 amino acids near the N‐terminal end of the sucrose‐specific porin ScrY causes its functional similarity to LamB in vivo and in vitro
Author(s) -
Schülein Katrin,
Andersen Christian,
Benz Roland
Publication year - 1995
Publication title -
molecular microbiology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.857
H-Index - 247
eISSN - 1365-2958
pISSN - 0950-382X
DOI - 10.1111/j.1365-2958.1995.mmi_17040757.x
Subject(s) - porin , biology , mutant , biochemistry , amino acid , translocase , membrane , wild type , escherichia coli , peptide sequence , lipid bilayer , glutamine , microbiology and biotechnology , bacterial outer membrane , biophysics , gene , chromosomal translocation
A deletion mutant ScrΔ3‐73 of the sucrose‐specific porin ScrY was constructed in which 70 amino acids of the mature protein were deleted near the N‐terminal end. ScrYΔ3‐72 was still able to oligomerize and inserted properly into the outer membrane of an Escherichia coli strain. The protein was isolated and purified by standard procedures. The mutant protein showed, in contrast to wild‐type ScrY, a tight association with the murein. Reconstitution experiments with artificial lipid bilayer membranes demonstrated that ScrYΔ3‐72 produced defined, cation‐selective channels in planar lipid bilayers. Its single‐channel conductance was reduced to about half of the value of wild‐type ScrY. The deletion had a relatively small influence on the stability constants for carbohydrate binding. However, in contrast to wild‐type ScrY, [ 14 C]‐maltopentaose was efficiently taken up into whole E. coli cells containing ScrYΔ3‐72. The sequence of the N‐terminus of mature ScrY was identified as starting with glutamine 23. The possible structure of ScrY and ScrYΔ3‐72 in the outer membrane is discussed.