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- Biocatalytic Properties and Substrate-binding Ability of a Modular GH10 β-1,4-Xylanase from an Insect-symbiotic Bacterium, Streptomyces mexicanus HY-14
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Do Young Kim , Dong-Ha Shin , Sora Jung , Jong Suk Lee , Han-Young Cho , Kyung Sook Bae , Chang-Keun Sung , Young Ha Rhee , Kwang-Hee Son , Ho-Yong Park
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J. Microbiol. 2014;52(10):863-870. Published online October 1, 2014
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DOI: https://doi.org/10.1007/s12275-014-4390-8
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Abstract
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The gene (1350-bp) encoding a modular β-1,4-xylanase (XylU),
which consists of an N-terminal catalytic GH10 domain and
a C-terminal carbohydrate-binding module 2 (CBM 2), from
Streptomyces mexicanus HY-14 was cloned and functionally
characterized. The purified His-tagged recombinant enzyme
(rXylU, 44.0 kDa) was capable of efficiently hydrolyze diverse
xylosidic compounds, p-nitrophenyl-cellobioside, and pnitrophenyl-
xylopyranoside when incubated at pH 5.5 and
65°C. Especially, the specific activities (649.8 U/mg and 587.0
U/mg, respectively) of rXylU toward oat spelts xylan and
beechwood xylan were relatively higher than those (<500.0
U/mg) of many other GH10 homologs toward the same
substrates. The results of enzymatic degradation of birchwood
xylan and xylooligosaccharides (xylotriose to xylohexaose)
revealed that rXylU preferentially hydrolyzed the
substrates to xylobiose (>75%) as the primary degradation
product. Moreover, a small amount (4%<) of xylose was detected
as the degradation product of the evaluated xylosidic
substrates, indicating that rXylU was a peculiar GH10 β-1,4-
xylanase with substrate specificity, which was different from
its retaining homologs. A significant reduction of the binding
ability of rXylU caused by deletion of the C-terminal CBM
2 to various insoluble substrates strongly suggested that the
additional domain might considerably contribute to the
enzyme-substrate interaction.
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Citations
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