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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

Production, purification and biochemical characterization of dextransucrase from Lactic acid bacteria isolated from sauerkraut

TL;DR: In this article, Lactobacillus sp has been isolated form saerkraut for the production of dextransucrase and the results showed that the enzyme exhibited Vmax plusmn mu mole min Km plusmn mg ml and Kcat s.
Journal ArticleDOI

Utilization of agro-industrial by-products as substrates for dextransucrase production by Leuconostoc mesenteroides T3: Process optimization using response surface methodology

TL;DR: In this paper, the potential of distillery stillage combined with sugar beet molasses, supplemented with sucrose and manganese to be employed as a valuable medium growth for lactic acid bacteria and production of DS was revealed.

Producción e inmovilización de la enzima dextransacarasa (DS) producida por Leuconostoc mesenteroides para la biosíntesis de dextrano.

Abstract: El grupo de Biopolimeros y Biofuncionales del Instituto de Biotecnologia ha trabajado en optimizar las condiciones para la produccion de la enzima dextransacarasa empleada para la produccion del dextrano. El objetivo de este trabajo consistio en evaluar la produccion e inmovilizacion de la enzima dextransacarasa (DS), producida por una cepa nativa colombiana de Leuconostoc mesenteroides IBUN 91.2.98 por fermentacion empleando un medio modificado de sacarosa al 6%, con una concentracion de fosfatos 0,1 M, pH 7,2 no controlado, temperatura de 30°C, agitacion 150 r.p.m y a un tiempo de fermentacion de 4 horas. La actividad enzimatica se evaluo mediante la determinacion de azucares reductores por el metodo DNS (acido 3,5 Dinitrosalicilico) y glucosa por el metodo de glucosa oxidasa, obteniendose una actividad hidrolitica de 4,8 a 7,3 U/ml y de transferencia de 4,3 a 7 U/ml. El peso molecular aproximado de la enzima determinada por electroforesis de proteinas (SDS-PAGE) fue aproximadamente de 178 a 180 kDa. La DS se inmovilizo mediante dos metodos: adsorcion en Sephadex G-100 y union covalente a Eupergit CM, obteniendo una actividad hidrolitica baja de 0,051 U/ml para Sephadex G-100 y 0,052 U/ml para el Eupergit CM. La actividad de transferencia no se pudo determinar.

김치로부터 분리된 Leuconostoc sp. strain YSK 균주에 의한 덱스트란 생산 조건의 최적화

TL;DR: In this article, a bacterium producing non-or partially digestible dextran was isolated from kimchi broth by enrichment culture technique and identified tentatively as Leuconostoc sp. strain SKY.
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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