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液体培养可提高香菇营养缺陷型菌株(ser(-))原生质体的形成率。

Liquid culture enhances protoplast formation from the auxotroph (ser(-)) ofLentinula edodes.

作者信息

Kim C, Kim B K

机构信息

Department of Microbial Chemistry, College of Pharmacy, Seoul National University, 151-742, Seoul, Korea.

出版信息

Arch Pharm Res. 1997 Jun;20(3):206-11. doi: 10.1007/BF02976146.

Abstract

The optimal conditions for the production and regeneration of the protoplasts fromLentinula edodes were studied. Protoplast formation from the mycelia ofL. edodes which were cultured in liquid medium showed a significantly high yield compared with that of the mycelia which were cultured on cellophane covered agar media. A mixture of Novozyme 234 (15 mg/ml) and Cellulase Onozuka R10 (10 mg/ml) in 0.6 M mannitol (pH 4) was optimal lytic enzyme for the protoplast release. The optimal incubation time and mycelia age were 3.5-4 hours at 30 degrees C and 6-8 days, respectively. Regeneration frequency was 0.18% plated onto a medium containing 0.6 M sucrose, and 0.08% plated onto a medium containing mannitol. But hardly any regeneration was observed in the media containing NaCl, KCl, or MgSO(4). More than 90% of the protoplasts contianed nuclei and the nucleus number per protoplast was 1.1. The DNA content per nucleus was 5.1 pg. The diameter of the protoplast was 3-5 mum and it had a well defined cell structure.

摘要

研究了香菇原生质体产生和再生的最佳条件。与在覆盖有玻璃纸的琼脂培养基上培养的香菇菌丝体相比,在液体培养基中培养的香菇菌丝体形成原生质体的产量显著更高。在0.6M甘露醇(pH4)中,Novozyme 234(15mg/ml)和纤维素酶Onozuka R10(10mg/ml)的混合物是释放原生质体的最佳裂解酶。最佳孵育时间和菌丝体年龄分别为30℃下3.5 - 4小时和6 - 8天。接种到含有0.6M蔗糖的培养基上的再生频率为0.18%,接种到含有甘露醇的培养基上的再生频率为0.08%。但在含有NaCl、KCl或MgSO₄的培养基中几乎未观察到再生。超过90%的原生质体含有细胞核,每个原生质体的细胞核数为1.1个。每个细胞核的DNA含量为5.1pg。原生质体直径为3 - 5μm,具有明确的细胞结构。

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