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Isolation of a Novel Gellan-Depolymerizing Bacillus sp. Strain YJ-1
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  • Isolation of a Novel Gellan-Depolymerizing Bacillus sp. Strain YJ-1
저자명
Jung. Yu-Jin,Park. Cheon-Seok,Lee. Hyeon-Gyu,Cha. Jae-Ho
간행물명
Journal of microbiology and biotechnology
권/호정보
2006년|16권 12호|pp.1868-1873 (6 pages)
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한국미생물생명공학회
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이 논문은 한국과학기술정보연구원과 논문 연계를 통해 무료로 제공되는 원문입니다.
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기타언어초록

A novel microorganism that could degrade high molecular weight gellan was screened and isolated from soil. On gellan plate, the microorganism grew well and completely liquefied the plate. The gellan-degrading microorganism was isolated by pure culture on glucose and nutrient agar medium afterwards. The 16S rDNA sequence analysis and biochemical tests using an API 50CHB/20E kit revealed that the strain belonged to Bacillus sp. The isolate, named as Bacillus sp. YJ-1, showed optimum gellan-degrading activity in 0.5% gellan medium at pH 7.5 and 37$^{circ}C$. The activity was measured and evaluated by the thiobarbituric acid and thin-layer chromatography method. Mass spectrometry revealed that the major gellan.. depolymerized product was an unsaturated tetrasaccharide consisting of $Delta$4,5-glucuronic acid-(1$ ightarrow$4 )-$eta$-D-glucose-(1$ ightarrow$4)- $alpha$-L-rhamnose-(1$ ightarrow$3)-$eta$-D-glucose, which is a dehydrated repeating unit of gellan, thus the enzyme was identified as gellan lyase. When the gellan was present in the medium, the gellan-degrading activity was much higher than that in glucose-grown cells. These results indicate that in the presence of gellan, Bacillus sp. YJ-1 is able to metabolize the gellan by inducing gellan-degrading enzymes that can degrade gellan into small molecular weight oligosaccharides, and then the gellan. depolymerized products are taken up by the cells and utilized by intracellular enzymes.