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Cloning of a complementary DNA coding for the 100-kD antigenic protein of the PM-Scl autoantigen.

作者信息

Ge Q, Frank M B, O'Brien C, Targoff I N

机构信息

Arthritis and Immunology Program, Oklahoma Medical Research Foundation, Oklahoma City 73104.

出版信息

J Clin Invest. 1992 Aug;90(2):559-70. doi: 10.1172/JCI115895.

Abstract

Anti-PM-Scl antibodies are associated with polymyositis-scleroderma overlap or either disease alone. Among sera from 39 patients with anti-PM-Scl, 23 recognized the 100-kD band in immunoblot against HeLa cell extract, 16 of which also stained the 70-kD band. A human thymocyte lambda gt11 cDNA expression library was screened with anti-PM-Scl serum, and two clones were identified whose products reacted with 33 and 37 of 39 anti-PM-Scl sera, respectively, but none of 26 negative control sera. Affinity-purified antibody reacting specifically with plaques of the clone stained the 100-kD band on immunoblot, reacted with nucleoli of HEp-2 cells, and immunoprecipitated the PM-Scl protein complex. Partial sequences of both inserts were identical. One insert was fully sequenced, and additional 5' and 3' sequence was obtained using a gene-specific primer to form a cDNA with HeLa cell RNA as template followed by PCR. The complete nucleotide sequence included 2,739-bp coding for a predicted full-length protein of 98,088 D. There was no homology with the PM-Scl 75-kD protein and no significant homology with other proteins. A mixed-charge cluster was identified, with 22 charged amino acids of 37. In conclusion, the full-length cDNA sequence was determined coding for the PM-Scl 100-kD protein, the most commonly antigenic protein of the PM-Scl complex.

摘要
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/3022/443135/75547fd16194/jcinvest00051-0271-a.jpg

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