• Plant Resources
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• 제4권3호
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• pp.200-205
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• 2001

It was reported in our Previous paper that the fermented products from Gloeostereum incarnatum strongly inhibit the growth of six kinds of bacteria in human bodies. In this paper the appropriated conditions of immersing culture for the strain 8 903 of Gloeostereum incarnatum was analysed. And the output of the hypha and fermentative product was determined or compared. The prelimenaryresults showed that the appropriated conditions for the growth of Gloeostereum incarnatum are: (1)culture medium:glucose 3%; protein peoptne 0.2%; soybeancake power 1% yeast power 0.3%; KH2PO40.05%; MgSO4 0.03%; CaCO3 0.01%; vitamin Bl 0.001%; befor sterilization pH Value of six should be maintained; (2) temperature; 27f ~28f ; (3) time; about 200 hours; (4) ventilation; (30%∼50%)/min. The sigh of the end culture are: pH coming down about 4: remnant glucoses less 1%; amino nitrogens about 20%; time about eight days. In the aforementioned conditions, the output of fermentative product achieve to 2.5∼3g/L.

• 한국자원식물학회:학술대회논문집
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• 한국자원식물학회 2001년도 The 8th International Symposium
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• pp.74-82
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• 2001

It was reported in our Previous paper that the fermented products from Gloeostereum incarnatum strongly inhibit the growth of six kinds of bacteria in human bodies. In this paper the appropriated conditions of immersing culture for the strain 8 903 of Gloeostereum incarnatum was analysed. And the output of the hypha and fermentative product was determined or compared, The prelimenaryresults showed that the appropriated conditions for the growth of Gloeostereum incarnatum are: (1)culture medium:glucose 3%; protein peoptne 0.2%; soybeancake power 1%, yeast power 0.3%; KH2PO40.05%; MgSO4 0.03%; CaCO3 0.01%; vitamin Bl 0.001%; befor sterilization pH Value of six should be maintained; (2) temperature; 27$^{\circ}C$～28$^{\circ}C$; (3) time; about 200 hours; (4) ventilation; (30%～50%)/min. The sigh of the end culture we: pH coming down about 4: remnant glucoses less 1%, amino nitrogens about 20;, time about eight days. In the aforementioned conditions, the output of fermentative product achieve to 2.5 ～3g/L.

• 한국버섯학회지
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• 제12권2호
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• pp.107-116
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• 2014

본 연구에서는 느릅나무버섯의 자실체에서 메탄올과 열수를 이용해 추출한 물질의 항산화, 항염증 및 Melanoma B16/F10 세포에서의 멜라닌 생성 저해 효과를 탐색하였다. DPPH 라디칼 소거능과 환원력을 이용해 항산화 효과를 측정한 결과 양성대조군으로 사용한 BHT에 비해 항산화 효과는 낮았지만 다른 종류의 버섯에 비해 효과가 우수한 것으로 나타났으며, 철 이온 제거 항산화 실험에서 느릅나무버섯의 열수 추출물은 양성대조군인 BHT에 비해 철 이온을 효율적으로 제거하여 항산화 효과가 높게 나타났다. 느릅나무버섯 자실체의 염증 저해 실험에서는 배양 중인 RAW 264.7 대식세포에 자실체의 메탄올과 열수추출물을 각각 처리 한 후 염증 유도 물질인 LPS를 투여하여 추출물의 NO 생성 저해효과를 조사한 결과, 처리한 추출물의 농도 의존적으로 염증 유발의 주요 인자인 NO의 양이 현저하게 감소하는 우수한 소염효과를 보였으며, carrageenan에 의해 흰쥐 뒷발에 유도된 부종을 저해하는 실험에서는 투여한 추출물의 농도가 증가함에 따라 흰쥐의 뒷발에 유도된 부종의 용적도 비례적으로 감소하여 항염증 효과가 높은 것으로 나타났다. Melanoma 세포에 버섯추출물을 처리하고 생합성된 멜라닌의 양을 측정한 결과 농도 의존적으로 melanoma 세포내 멜라닌의 양이 감소하여 멜라닌 저해 효과가 높은 것으로 나타났다. 따라서 느릅나무버섯 자실체의 항산화, 항염증 및 멜라닌 생성 저해 선분은 앞으로 항산화제, 소염제 및 미백제로의 이용이 가능할 것으로 사료된다.

• Mycobiology
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• 제49권4호
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• pp.406-420
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• 2021

Gloeostereum incarnatum has edible and medicinal value and was first cultivated and domesticated in China. We sequenced the G. incarnatum monokaryotic strain GiC-126 on an Illumina HiSeq X Ten system and obtained a 34.52-Mb genome assembly sequence that encoded 16,895 predicted genes. We combined the GiC-126 genome with the published genome of G. incarnatum strain CCMJ2665 to construct a genetic linkage map (GiC-126 genome) that had 10 linkage groups (LGs), and the 15 assembly sequences of CCMJ2665 were integrated into 8 LGs. We identified 1912 simple sequence repeat (SSR) loci and detected 700 genes containing 768 SSRs in the genome; 65 and 100 of them were annotated with gene ontology (GO) terms and KEGG pathways, respectively. Carbohydrate-active enzymes (CAZymes) were identified in 20 fungal genomes and annotated; among them, 144 CAZymes were annotated in the GiC-126 genome. The A mating-type locus (MAT-A) of G. incarnatum was located on scaffold885 at 38.9 cM of LG1 and was flanked by two homeodomain (HD1) genes, mip and beta-fg. Fourteen segregation distortion markers were detected in the genetic linkage map, all of which were skewed toward the parent GiC-126. They formed three segregation distortion regions (SDR1-SDR3), and 22 predictive genes were found in scaffold1920 where three segregation distortion markers were located in SDR1. In this study, we corrected and updated the genomic information of G. incarnatum. Our results will provide a theoretical basis for fine gene mapping, functional gene cloning, and genetic breeding the follow-up of G. incarnatum.