Inderjit K. Dev
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Featured researches published by Inderjit K. Dev.
Journal of Bioenergetics and Biomembranes | 1990
Inderjit K. Dev; Paul H. Ray
AbstractSignal peptidases, the endoproteases that remove the amino-terminal signal sequence from many secretory proteins, have been isolated from various sources. Seven signal peptidases have been purified, two fromE. coli, two from mammalian sources, and three from mitochondrial matrix. The mitochondrial enzymes are soluble and function as a heterogeneous dimer. The mammalian enzymes are isolated as a complex and share a common glycosylated subunit. The bacterial enzymes are isolated as monomers and show no sequence homology with each other or the mammalian enzymes. The membrane-bound enzymes seem to require a substrate containing a consensus sequence following the −3, −1 rule of von Heijne at the cleavage site; however, processing of the substrate is strongly influenced by the hydrophobic region of the signal peptide. The enzymes appear to recognize an unknown three-dimensional motif rather than a specific amino acid sequence around the cleavage site. The matrix mitochondrial enzymes are metallo-endopeptidases; however, the other signal peptidases may belong to a unique class of proteases as they are resistant to chelators and most protease inhibitors. There are no data concerning the substrate binding site of these enzymes. In vivo, the signal peptide is rapidly degraded. Three different enzymes inEscherichia coli that can degrade a signal peptidein vitro have been identified. The intact signal peptide is not accumulated in mutants lacking these enzymes, which suggests that these peptidases individually are not responsible for the degredation of an intact signal peptidein vivo. It is speculated that signal peptidases and signal peptide hydrolases are integral components of the secretory pathway and that inhibition of the terminal steps can block translocation.
Biochemical and Biophysical Research Communications | 1991
Todd Talarico; Inderjit K. Dev; Philip J. Bassford; Paul H. Ray
Highly purified preparations of signal peptidase I (36 kDa) were found to undergo an apparent inter-autocatalytic degradation at 4 degrees C and 37 degrees C. The disappearance of the 36 kDa protein coincided with the stable appearance of a 31 kDa and a 5 kDa species. Amino-terminal sequencing of the 31 kDa product indicated a site specific cleavage following Ala38-Gln-Ala of signal peptidase I. The 31 kDa fragment was purified and shown to have 100-fold less activity than the native enzyme, with pre-maltose binding protein as a substrate.
Cancer Research | 1993
David S. Duch; Sheila D. Banks; Inderjit K. Dev; Scott Howard Dickerson; Robert Ferone; Louise S. Heath; Joan E. Humphreys; Vincent C. Knick; William Pendergast; Sara Singer; Gary K. Smith; Kathleen A. Waters; H. Robert Wilson
Journal of Bacteriology | 1992
W S Dallas; J E Gowen; Paul H. Ray; M J Cox; Inderjit K. Dev
Analytical Biochemistry | 1997
John T. Moore; Stephen T. Davis; Inderjit K. Dev
Journal of Medicinal Chemistry | 1991
Shu Wen Li; M. G. Nair; Donna M. Edwards; Roy L. Kisliuk; Y. Gaumont; Inderjit K. Dev; David S. Duch; Joan E. Humphreys; Gary K. Smith; Robert Ferone
Journal of Bacteriology | 1992
Todd Talarico; Paul H. Ray; Inderjit K. Dev; B M Merrill; W S Dallas
Journal of Medicinal Chemistry | 1993
William Pendergast; Jay V. Johnson; Scott Howard Dickerson; Inderjit K. Dev; David S. Duch; Robert Ferone; William R. Hall; Joan E. Humphreys; Joseph M. Kelly; David C. Wilson
Cancer Research | 1992
Gary K. Smith; David S. Duch; Inderjit K. Dev; Scott H. Kaufmann
Journal of Bacteriology | 1991
Todd Talarico; Inderjit K. Dev; W S Dallas; R Ferone; Paul H. Ray
