Affiliation:
1. Laboratoire Mayoly Spindler, Service Recherche, 78401 Chatou Cedex,1 and
2. Laboratoire de Microbiologie et Génétique Moléculaire, INRA-CNRS, 78850 Thiverval-Grignon,2 France
Abstract
ABSTRACT
We isolated the
LIP2
gene from the lipolytic yeast
Yarrowia lipolytica
. It was found to encode a 334-amino-acid precursor protein. The secreted lipase is a 301-amino-acid glycosylated polypeptide which is a member of the triacylglycerol hydrolase family (EC
3.1.1.3
). The Lip2p precursor protein is processed by the
KEX2
-like endoprotease encoded by
XPR6
. Deletion of the
XPR6
gene resulted in the secretion of an active but less stable proenzyme. Thus, the pro region does not inhibit lipase secretion and activity. However, it does play an essential role in the production of a stable enzyme. Processing was found to be correct in
LIP2
A
(multiple
LIP2
copy integrant)-overexpressing strains, which secreted 100 times more activity than the wild type, demonstrating that
XPR6
maturation was not limiting. No extracellular lipase activity was detected with the
lip2
knockout (KO) strain, strongly suggesting that extracellular lipase activity results from expression of the
LIP2
gene. Nevertheless, the
lip2
KO strain is still able to grow on triglycerides, suggesting an alternative pathway for triglyceride utilization in
Y. lipolytica
.
Publisher
American Society for Microbiology
Subject
Molecular Biology,Microbiology
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