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Abstract
ABC10alpha is a small polypeptide shared by the three yeast RNA polymerases. Homologous polypeptides in higher eukaryotes have a zinc-binding CX(2)C. CX(2)C motif and a conserved basic C-terminal end. These features are also found in archaeal gene products that may encode an RNA polymerase subunit. The CX(2)C. CX(2)C motif is partly dispensable, since only its first cysteine is essential for growth, whereas the basic C-terminal end is critical in vivo. A mutant in the latter domain has an RNA polymerase III-specific defect and, in vitro, impairs RNA polymerase III assembly. Polymerase activity was, however, not affected in various faithful transcription assays. The mutant is suppressed by a high gene dosage of the second largest subunit of RNA polymerase III, whereas the homologous subunits of RNA polymerase I and II have aggravating effects. In a two-hybrid assay, ABC10alpha binds to the C-terminal half of the second largest subunit of RNA polymerase I, in a way that requires the integrity of the CX(2)C. CX(2)C motif. Thus, ABC10alpha appears to interact directly with the second largest subunit during polymerase assembly. This interaction is presumably a major rate-limiting step in assembly, since diploid cells containing only one functional gene copy for ABC10alpha have a partial growth defect.
Highlights
Introduction of a uniqueSalI site after the stop codon of RPC10 in pGEN-RPC10␣ [12]
RPC10 is under the control of the pPGK1 promoter and can be excised by BamHI-SalI digestion
Halving the RPC10 Gene Dosage Has a Rate-limiting Effect on Growth—From previous work on yeast RNA pol I and pol III subunits (Refs. 31 and 32 and references therein), we know that deleting one gene copy in the corresponding diploid strains has no detectable effect on growth and that these gene deletions are fully recessive
Summary
Introduction of a uniqueSalI site after the stop codon of RPC10 in pGEN-RPC10␣ [12]. RPC10 is under the control of the pPGK1 promoter and can be excised by BamHI-SalI digestionDirectional cloning of a 2.2-kba BamHI-SalI fragment from pFL44L-RPC10 in pTSV31a [26]Directional cloning of a 0.26-kb BamHI-Bsp102I fragment from pGENs-RPC10 in pCM185 [49]. SalI site after the stop codon of RPC10 in pGEN-RPC10␣ [12]. RPC10 is under the control of the pPGK1 promoter and can be excised by BamHI-SalI digestion. Directional cloning of a 2.2-kba BamHI-SalI fragment from pFL44L-RPC10 in pTSV31a [26]. Directional cloning of a 0.26-kb BamHI-Bsp102I fragment from pGENs-RPC10 in pCM185 [49]. Derivative of pGENs-RPC10 containing an Nterminal HA-tagged form of RPC10. Derivative of pGEN-rpc containing an Nterminal HA-tagged rpc. Directional cloning of a 5.7-kb KpnI-SalI fragment bearing RBP2 in pFL44L. Directional cloning of a 1.1-kb SacI-SalI fragment bearing RPB5 in pFL44L. Directional cloning of a 1.5-kb BamHI-XhoI fragment bearing RPB6, inserted between the BamHI and SalI sites of pFL44L. Directional cloning of a 2.5-kb SacI-SalI fragment bearing RPB8 in pF44L
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