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Molecular cloning of a gene coding for thermostable beta-glucanase from Bacillus macerans

✍ Scribed by Dr. Rainer Borriss; Renate Manteuffel; Jürgen Hofemeister

Publisher
John Wiley and Sons
Year
1988
Tongue
English
Weight
505 KB
Volume
28
Category
Article
ISSN
0233-111X

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✦ Synopsis

The bglM gene DNA coding for a thermostable beta-I .3,1.4-glucanase of Bacillus maceruns E I38 was isolated by direct shot-gun cloning into Escherirhia coli using plasmid pBR322 as a vector. By deletion analysis the bg/M coding region was located within a 1.0 kb region of the cloned Bacillus DNA fragment. In E. coli, plasmid pBGLM12/2 containing the B. macerans bg/M gene gave rise to a beta-glucanase expression 40 times higher than that of the B. macerans gene donor. The molecular weight of beta-glucanase, isolated either from E. coli cells or from the culture filtrate of B. maceruns, was in the range of 24 kD. The enzymes purified from E. coli or from the culture filtrate of B. macerans, had a halflife of about 40 min at 65 "C. This indicated an increased temperature stability of the B. mncerans enzyme in comparison to other Bacillus-beta-glucanases.

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