Abstract
A novel ribosomal S6 kinase, termed p70 S6 kinase beta (p70beta), which has a highly conserved amino acid sequence compared with that of p70/p85 S6 kinase (p70alpha) within the catalytic, kinase extension, and autoinhibitory pseudosubstrate domains, was identified. However, the amino acid sequence of p70beta differs from that of p70alpha in the noncatalytic amino-terminal region and in the carboxyl-terminal tail, which contains a proline-rich region. The majority of the regulatory phosphorylation sites identified in p70alpha are conserved in p70beta. Two isoforms of p70beta, referred to as beta1 (495 amino acids) and beta2 (482 amino acids), could be expressed from the single gene either by alternative mRNA splicing or by the use of alternative start codons. Here we report the characterization of p70beta2. Similarly to p70alpha, the catalytic activity of p70beta toward ribosomal protein S6 could be rapidly activated by serum, insulin, and phorbol ester in transiently transfected cells. The p70beta kinase was found to be significantly less sensitive to wortmannin and rapamycin than p70alpha. These results indicate that p70beta has the potential to participate in the regulation of protein synthesis and the cell cycle.
Highlights
In addition to the role of p70␣ in protein synthesis, it has been shown that p70 S6 kinase is required during the G1 phase of the cell cycle [6, 8]
Among fractions of serum-treated HEK293 cells separated using an anion exchange column, we detected several immunoreactive bands that were recognized by immunoblotting with the anti-pS434 Ab in a rapamycinsensitive manner but were not detected with the anti-p70␣C Ab. These data indicated that p70 S6 kinase isoforms may exist in which the Ser434 site is conserved but that do not have a sequence homologous to the carboxyl-terminal end of p70␣. These results prompted us to search for sequences that could encode mammalian isoforms of p70 S6 kinase in the expressed sequence tag (EST) data bases
The full-length cDNA clone corresponding to the identified EST clones was isolated from a library of HEK293 cells using the insert of EST clone AA410355 as a probe
Summary
These observations suggested to us that isoforms of p70 S6 kinase, other than p70␣, exist and prompted a search of the expressed sequence tag (EST) data base that revealed potentially novel isoforms of p70 S6 kinase. Construction of Plasmids and Expression of GST Fusion Protein—The full-length coding sequence corresponding to p702 (amino acids 14 – 495 of p701) was amplified by polymerase chain reaction using the clone 53 as a template and cloned into the pcDNA1 vector (Invitrogen) in-frame with the amino-terminal FLAG epitope.
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