Isolation and characterization of full-length cDNA clones for human alpha-, beta-, and gamma-actin mRNAs: skeletal but not cytoplasmic actins have an amino-terminal cysteine that is subsequently removed.

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Mol Cell Biol. 1983 May; 3(5): 787-795

Isolation and characterization of full-length cDNA clones for human alpha-, beta-, and gamma-actin mRNAs: skeletal but not cytoplasmic actins have an amino-terminal cysteine that is subsequently removed.

P Gunning, P Ponte, H Okayama, J Engel, H Blau and L Kedes

ABSTRACT

cDNA clones encoding three classes of human actins have beenisolated and characterized. The first two classes (gamma andbeta, cytoplasmic actins) were obtained from a cDNA libraryconstructed from simian virus 40-transformed human fibroblastmRNA, and the third class (alpha, muscle actin) was obtainedfrom a cDNA library constructed from adult human muscle mRNA.A new approach was developed to enrich for full-length cDNAs.The human fibroblast cDNA plasmid library was linearized withrestriction enzymes that did not cut the inserts of interest;it was then size-fractionated on gels, and the chimeric moleculesof optimal length were selected for retransformation of bacteria.When the resulting clones were screened for actin-coding sequencesit was found that some full-length cDNAs were enriched as muchas 50- to 100-fold relative to the original frequency of full-lengthclones in the total library. Two types of clones were distinguished.One of these clones encodes gamma actin and contains 100 basepairs of 5' untranslated region, the entire protein coding region,and the 3' untranslated region. The second class encodes betaactin, and the longest such clone contains 45 base pairs of5' untranslated region plus the remainder of the mRNA extendingto the polyadenylic acid tail. A third class, obtained fromthe human muscle cDNA library, encodes alpha actin and contains100 base pairs of 5' untranslated region, the entire codingregion, and the 3' untranslated region. Analysis of the DNAsequences of the 5' end of the clones demonstrated that althoughbeta- and gamma-actin genes start with a methionine codon (MET-Asp-Asp-Aspand MET-Glu-Glu-Glu, respectively), the alpha-actin gene startswith a methionine codon followed by a cysteine codon (MET-CYS-Asp-Glu-Asp-Glu).Since no known actin proteins start with a cysteine, it is likelythat post-translational removal of cysteine in addition to methionineaccompanies alpha-actin synthesis but not beta- and gamma-actinsynthesis. This observation has interesting implications bothfor actin function and actin gene regulation and evolution.

Mol Cell Biol. 1983 May; 3(5): 787-795

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