The domain within your query sequence starts at position 10 and ends at position 154; the E-value for the Creatinase_N domain shown below is 5.2e-15.
LRQLRQAMRNSEYVAEPIQAYIIPSGDAHQSEYIAPCDCRRAFVSGFDGSAGTAIITEEH AAMWTDGRYFLQAAKQMDNNWTLMKMGLKDTPTQEDWLVSVLPEGSRVGVDPLIIPTDYW KKMAKVLRSAGHHLVPVKENLVDKI
Creatinase_N |
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PFAM accession number: | PF01321 |
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Interpro abstract (IPR000587): | Creatinase or creatine amidinohydrolase ( EC 3.5.3.3 ) catalyses the conversion of creatine and water to sarcosine and urea. The enzyme works as a homodimer, and is induced by choline chloride. Each monomer of creatinase has two clearly defined domains, a small N-terminal domain, and a large C-terminal domain. The structure of the C-terminal region represents the "pita-bread" fold. The fold contains both alpha helices and an anti-parallel beta sheet within two structurally similar domains that are thought to be derived from an ancient gene duplication. The active site, where conserved, is located between the two domains. The fold is common to methionine aminopeptidase ( EC 3.4.11.18 ), aminopeptidase P ( EC 3.4.11.9 ), prolidase ( EC 3.4.13.9 ), agropine synthase and creatinase ( EC 3.5.3.3 ). Though many of these peptidases require a divalent cation, creatinase is not a metal-dependent enzyme [ (PUBMED:8146141) (PUBMED:12136144) (PUBMED:8471602) ]. |
GO function: | hydrolase activity (GO:0016787) |
This is a PFAM domain. For full annotation and more information, please see the PFAM entry Creatinase_N