AI Article Synopsis

  • Previous studies found that the Atlantic cod genome has unusual immune system gene variations, leading this study to analyze lysozyme activity and gene distribution in cod.
  • Enzymatic tests confirmed the presence of g-type lysozymes but surprisingly revealed no c-type lysozymes, with unsuccessful searches for their genes in cod.
  • Four g-type lysozyme genes were identified, showing different expression levels across cod organs and varying responses to bacterial infections, highlighting the cod's unique immune adaptations due to the absence of c-type lysozymes.

Article Abstract

Previous analyses of the Atlantic cod genome showed unique combinations of lacking and expanded number of genes for the immune system. The present study examined lysozyme activity, lysozyme gene distribution and expression in cod. Enzymatic assays employing specific bacterial lysozyme inhibitors provided evidence for presence of g-type, but unexpectedly not for c-type lysozyme activity. Database homology searches failed to identify any c-type lysozyme gene in the cod genome or in expressed sequence tags from cod. In contrast, we identified four g-type lysozyme genes (LygF1a-d) constitutively expressed, although differentially, in all cod organs examined. The active site glutamate residue is replaced by alanine in LygF1a, thus making it enzymatic inactive, while LygF1d was found in two active site variants carrying alanine or glutamate, respectively. In vitro and in vivo infection by the intracellular bacterium Francisella noatunensis gave a significantly reduced LygF1a and b expression but increased expression of the LygF1c and d genes as did also the interferon gamma (IFNγ) cytokine. These results demonstrate a lack of c-type lysozyme that is unprecedented among vertebrates. Our results further indicate that serial gene duplications have produced multiple differentially regulated cod g-type lysozymes with specialised functions potentially compensating for the lack of c-type lysozymes.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC4914998PMC
http://dx.doi.org/10.1038/srep28318DOI Listing

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