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Open AccessJournal ArticleDOI

The effect of certain cultural factors on production of dextransucrase by Leuconostoc mesenteroides.

TLDR
Observation on factors affecting production of dextransucrase from Leuconostoc mesenteroides, strain NRRL B-512 and the possibility that more than one enzyme may be involved in the synthesis ofdextran is recognized.
Abstract
Present knowledge on the characteristics of dextransucrase and its mode of action is based primarily on the important investigations of Hehre (1941, 1946, 1951) and Hehre and Sugg (1942). Hitherto, a serious impediment to studies of this interesting enzyme has been the difficulty of procuring dextransucrase. Development of further knowledge about it would be greatly facilitated by the availability of culture liquors rich in dextransucrase. The rapid formation of dextransucrase in high yields has been reported in a preliminary note (Koepsell and Tsuchiya, 1952). The present report deals in greater detail with our observations on factors affecting production of dextransucrase from Leuconostoc mesenteroides, strain NRRL B-512.2 However, culture liquors high in activity have been obtained from a large number of the organisms tested. The dextran produced by strain NRRL B-512 in the conventional whole culture procedure contains about 95 per cent a-1,6-glucopyranosidic linkage. Although the non-1,6 linkages have been assumed to be of the a-1,4 type, definite proof on this point is lacking (Jeanes and Wilham, 1950). L. mesenteroides, strain NRRL B-512, or its substrains, is the organism principally used in investigations of clinical dextran in the United States. Although the term \"dextransucrase\" is used in the singular for convenience, the possibility that more than one enzyme may be involved in the synthesis of dextran is recognized.

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Journal ArticleDOI

Dextran synthesized by Leuconostoc mesenteroides BD1710 in tomato juice supplemented with sucrose

TL;DR: The results showed that the polysaccharide synthesized by L. mesenteroides BD1710 in the tomato-juice-sucrose medium was dextran with a peak molecular weight of 6.35 × 10(5)Da, a linear backbone composed of consecutive α-(1 → 6)-linked d-glucopyranosyl units and approximately 6% α-( 1 → 3) branches.
Journal ArticleDOI

Effect of phosphate concentration on the production of dextransucrase by Leuconostoc mesenteroides NRRL B512F.

TL;DR: A study about the effect of phosphate concentration on cell propagation in a semicontinuous shake-flask culture is described, and an increase on biomass and on the enzyme activity was found when phosphate enriched medium was used.
Journal ArticleDOI

Dextran synthesis by immobilized dextran sucrase.

TL;DR: The enzyme preparation has been concentrated from the fermentation broth by ultrafiltration and purified by gel permeation chromatography on Ultrogel, and the specific activity of the dextran sucrase was greatly enhanced by calcium chloride addition to the purified enzyme.
Journal ArticleDOI

Identification, effective purification and functional characterization of dextransucrase from Leuconostoc mesenteroides NRRL B-640

TL;DR: The extracellular dextransucrase from Leuconostoc mesenteroides NRRL B-640 was purified using polyethylene glycol fractionation (PEG) and gel-filtration and confirmed the presence of dextran, when run on SDS-PAGE under non-denaturing gels for in situ activity detection by Periodic Acid Schiff's staining.
References
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Journal ArticleDOI

Enzymatic synthesis of dextran

TL;DR: A study of acceptor specificity in dextran synthesis was undertaken with the object of elucidating the polymerization mechanism and it was hoped that clues leading to the direct enzymatic synthesis of “clinical” dextransucrase with an average molecular weight in the range of 50,000 to 100,000 would be found.
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