Use of a cDNA clone for the fourth component of human complement (C4) for analysis of a genetic deficiency of C4 in guinea pig.

Abstract

A c[complementary]DNA clone for the 4th complement component (C4), pC4AL1, was isolated from a human adult liver cDNA library by using a synthetic oligonucleotide mixture containing all 384 possible sequences coding for residues 14-21 of the C4 .gamma.-chain amino acid sequence. This clone spans the entire C4 .gamma.-chain coding sequence and includes a short 3'' untranslated region, a poly(A) recognition site, and 16 nucleotides of the poly(A) tail. The 5'' end of the clone begins 18 nucleotides upstream from the amino terminus of the C4 .gamma. chains and codes for Arg-Asn-Arg-Arg-Arg-Arg, a highly charged proteolytic cleavage site involved in the processing of pro-C4 to native C4. Liver mRNA preparations from C4-deficient guinea pigs were incapable of directing synthesis of pro-C4 or C4 peptides in cell-free translation experiments. Southern blot analysis using pC4AL1 as a hybridization probe of C4-deficient guinea pig DNA established that the deficiency is not the result of deletion of the entire C4 gene. RNA blot analysis using pC4AL1 as a hybridization probe of normal guinea pig liver mRNA revealed a C4 mRNA of 5.0 kilobases (kb). No such mRNA species was observed in C4-deficient guinea pig liver mRNA; however, a 7.0-kb RNA was detected, indicating the presence of a C4 precursor RNA. The basis of C4 deficiency in the guinea pig may be a post-transcriptional defect in the processing of C4 precursor RNA to mature C4 mRNA.