TY - JOUR
T1 - Structure-activity determinants in paneth cell α-defensins
T2 - Loss-of-function in mouse cryptdin-4 by charge-reversal at arginine residue positions
AU - Tanabe, Hiroki
AU - Qu, Xiaoqing
AU - Weeks, Colby S.
AU - Cummings, Jason E.
AU - Kolusheva, Sofiya
AU - Walsh, Kevin B.
AU - Jelinek, Raz
AU - Vanderlick, T. Kyle
AU - Selsted, Michael E.
AU - Ouellette, Andre J.
PY - 2004/3/19
Y1 - 2004/3/19
N2 - Paneth cells secrete microbicidal enteric α-defensins into the small intestinal lumen, and cryptdin-4 (Crp4) is the most bactericidal of the mouse α-defensin peptides in vitro. Here, site-directed Arg to Asp mutations in Crp4 have been shown to attenuate or eliminate microbicidal activity against all of the bacterial species tested regardless of the Arg residue position. R31D/R32D charge-reversal mutagenesis at the C terminus and mutations at R16D/R18D, R16D/R24D, and R18D/R24D in the Crp4 polypeptide chain eliminated in vitro bactericidal activity, blocked peptide-membrane interactions, as well as Crp4-mediated membrane vesicle disruption. Lys for Arg charge-neutral substitutions in (R16K/R18K)-Crp4 did not alter the bactericidal activity relative to Crp4, showing that bactericidal activity appears not to require the guanidinium side chain of Arg at those two positions. Partial restoration of (R31D/R32D)-Crp4 bactericidal activity occurred when an electropositive Arg for Gly substitution was introduced at the peptide N terminus and the (G1R/R31D/R32D)-Crp4 peptide exhibited intermediate membrane binding capability. Also, the loss of peptide bactericidal activity in (G1D/R31D/ R32D)-Crp4 and (R16D/R24D)-Crp4 mutants corresponded with diminished phospholipid vesicle disruptive activity. Fluorophore leakage from anionic phospholipid vesicles induced by the charge-reversal variants was negligible relative to Crp4 and lower than that induced by pro-Crp4, the inactive Crp4 precursor. Thus, Arg residues function as determinants of Crp4 bactericidal activity by facilitating or enabling target cell membrane disruption. The role of the Arg residues, however, was surprisingly independent of their position in the polypeptide chain.
AB - Paneth cells secrete microbicidal enteric α-defensins into the small intestinal lumen, and cryptdin-4 (Crp4) is the most bactericidal of the mouse α-defensin peptides in vitro. Here, site-directed Arg to Asp mutations in Crp4 have been shown to attenuate or eliminate microbicidal activity against all of the bacterial species tested regardless of the Arg residue position. R31D/R32D charge-reversal mutagenesis at the C terminus and mutations at R16D/R18D, R16D/R24D, and R18D/R24D in the Crp4 polypeptide chain eliminated in vitro bactericidal activity, blocked peptide-membrane interactions, as well as Crp4-mediated membrane vesicle disruption. Lys for Arg charge-neutral substitutions in (R16K/R18K)-Crp4 did not alter the bactericidal activity relative to Crp4, showing that bactericidal activity appears not to require the guanidinium side chain of Arg at those two positions. Partial restoration of (R31D/R32D)-Crp4 bactericidal activity occurred when an electropositive Arg for Gly substitution was introduced at the peptide N terminus and the (G1R/R31D/R32D)-Crp4 peptide exhibited intermediate membrane binding capability. Also, the loss of peptide bactericidal activity in (G1D/R31D/ R32D)-Crp4 and (R16D/R24D)-Crp4 mutants corresponded with diminished phospholipid vesicle disruptive activity. Fluorophore leakage from anionic phospholipid vesicles induced by the charge-reversal variants was negligible relative to Crp4 and lower than that induced by pro-Crp4, the inactive Crp4 precursor. Thus, Arg residues function as determinants of Crp4 bactericidal activity by facilitating or enabling target cell membrane disruption. The role of the Arg residues, however, was surprisingly independent of their position in the polypeptide chain.
UR - http://www.scopus.com/inward/record.url?scp=12144289841&partnerID=8YFLogxK
U2 - 10.1074/jbc.M310251200
DO - 10.1074/jbc.M310251200
M3 - Article
AN - SCOPUS:12144289841
SN - 0021-9258
VL - 279
SP - 11976
EP - 11983
JO - Journal of Biological Chemistry
JF - Journal of Biological Chemistry
IS - 12
ER -