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Publication : Molecular cloning of mouse allantoicase cDNA.

First Author  Vigetti D Year  2001
Journal  Biochim Biophys Acta Volume  1519
Issue  1-2 Pages  117-21
PubMed ID  11406280 Mgi Jnum  J:70053
Mgi Id  MGI:2136123 Doi  10.1016/s0167-4781(01)00207-x
Citation  Vigetti D, et al. (2001) Molecular cloning of mouse allantoicase cDNA. Biochim Biophys Acta 1519(1-2):117-21
abstractText  The uric acid degradation pathway is progressively lost during vertebrate evolution. In mammals, the end product of this catabolic pathway is allantoin and, therefore, no allantoicase should be present in mouse tissues. Surprisingly, we have found an expressed sequence tag (EST) from mouse testis with high similarity to allantoicase. To characterize this transcript, we have completely sequenced the corresponding EST clone insert and found a 1495 bp long cDNA coding for a 414 amino acid long protein. Identities of mouse versus microorganism allantoicases range from 25 to 30%. Identity reaches 54% when compared to Xenopus allantoicase. Among the tested tissues, only testis possesses the allantoicase transcript. Although no deleterious mutations were found in the coding region, no allantoicase activity could be detected in mouse testis.
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