Dominant mutations in a gene encoding a putative protein kinase (BCK1) bypass the requirement for a Saccharomyces cerevisiae protein kinase C homolog.

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Mol Cell Biol. 1992 January; 12(1): 172-182

Dominant mutations in a gene encoding a putative protein kinase (BCK1) bypass the requirement for a Saccharomyces cerevisiae protein kinase C homolog.

K S Lee and D E Levin

Department of Biochemistry, Johns Hopkins University School of Hygiene and Public Health, Baltimore, Maryland 21205.

ABSTRACT

The PKC1 gene of Saccharomyces cerevisiae encodes a homologof mammalian protein kinase C that is required for yeast cellgrowth and division. To identify additional components of thepathway in which PKC1 functions, we isolated extragenic suppressorsof a pkc1 deletion mutant. All of the suppressor mutations weredominant for suppressor function and defined a single locus,which was designated BCK1 (for bypass of C kinase). A molecularclone of one suppressor allele, BCK1-20, was isolated on a centromere-containingplasmid through its ability to rescue a conditional pkc1 mutant.The BCK1 gene possesses a 4.4-kb uninterrupted open readingframe predicted to encode a 163-kDa protein kinase. The BCK1gene product is not closely related to any known protein kinase,sharing only 45% amino acid identity with its closest knownrelative (the STE11-encoded protein kinase) through a regionrestricted to its putative C-terminal catalytic domain. Deletionof BCK1 resulted in a temperature-sensitive cell lysis defect,which was suppressed by osmotic stabilizing agents. Becausepkc1 mutants also display a cell lysis defect, we suggest thatPKC1 and BCK1 may normally function within the same pathway.Suppressor alleles of BCK1 differed from the wild-type genein a region surrounding a potential PKC phosphorylation siteimmediately upstream of the predicted catalytic domain. Thisregion may serve as a hinge between domains whose interactionis regulated by PKC1.

Mol Cell Biol. 1992 January; 12(1): 172-182

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