STRUCTURAL ORGANIZATION OF THE GENE ENCODING THE RAT PANCREATITIS-ASSOCIATED PROTEIN - ANALYSIS OF ITS EVOLUTIONARY HISTORY REVEALS AN ANCIENT DIVERGENCE FROM THE OTHER CARBOHYDRATE-RECOGNITION DOMAIN-CONTAINING GENES

Rat pancreatitis-associated protein (PAP) mRNA is barely detectable in normal pancreas and overexpressed during acute pancreatitis (Iovanna, J., Orelle, B., Keim, V., and Dagorn J.-C. (1991) J. Biol. Chem. 266, 24664-24669). RNA amplification by reverse-transcriptase-coupled poly merase chain reaction showed that PAP mRNA was constitutively expresse d in duodenum, jejunum, and ileum, at similar levels as in pancreas du ring the acute phase of pancreatitis. A weak expression was also detec ted in several other tissues. The rat PAP gene was isolated from a gen omic library and characterized over 3.2 kilobases of gene sequence and 1.2 kilobases of 5'-flanking sequence. The 5' end of the coding seque nce was determined by primer extension of the PAP transcript. Several potential regulatory elements were identified in the promoter region, including a pancreas-specific consensus sequence, two Pan1 (pancreas-s pecific) transcription activators, two IL-6 response elements, and one glucocorticoid response element. The PAP coding sequence spanned over six exons. The first three exons encoded the 5'-untranslated region o f the mRNA, the signal peptide, and 39 amino acids of the NH2-terminal end of the mature protein, respectively. The other three exons encode d a domain of the protein with significant homology to the carbohydrat e-recognition domain of animal lectins. Sequence comparison of the PAP gene with 13 carbohydrate-recognition domain-containing genes reveale d that they derived from the same ancestor gene. Position of introns w ithin the carbohydrate-recognition domain were different, however, sug gesting that PAP belongs to a new group of lectins. These results supp ort the hypothesis that genes encoding PAP and other lectins evolved f rom a common ancestor gene by intron gain.