Bile-salt activated lipase (BAL) is a pancreatic enzyme
that digests a variety of lipids in the small intestine.
A distinct property of BAL is its dependency on bile salts
in hydrolyzing substrates of long acyl chains or bulky
alcoholic motifs. A crystal structure of the catalytic
domain of human BAL (residues 1–538) with two surface
mutations (N186D and A298D), which were introduced in attempting
to facilitate crystallization, has been determined at 2.3
Å resolution. The crystal form belongs to space group
P212121 with one monomer
per asymmetric unit, and the protein shows an α/β
hydrolase fold. In the absence of bound bile salt molecules,
the protein possesses a preformed catalytic triad and a
functional oxyanion hole. Several surface loops around
the active site are mobile, including two loops potentially
involved in substrate binding (residues 115–125 and
270–285).