细胞培养进口血清进口胎牛血清进口新生牛血清进口猪血清马血清- 支原体检测盒及标准品常规PCR检测试剂盒荧光定量PCR检测(qPCR法)支原体DNA提取灵敏度标准品(方法验证用)特异性标准品(方法验证用)PCR定量标准品(可用于方法验证)
支原体祛除试剂细胞中支原体祛除环境支原体祛除水槽支原体祛除
干细胞培养基- DNA/RNA污染祛除DNA/RNA污染祛除试剂DNA污染监测
- RNA病毒研究试剂RNA病毒检测试剂盒病毒RNA提取
- PCR仪器及配套产品DNA污染监测祛除PCR/qPCR仪性能检查PCR试剂PCR试剂盒PCR预混液(冻干粉)热启动聚合酶MB Taq DNA
- 微生物PCR检测食品检测类产品食品微生物检测细菌PCR检测
细胞培养进口血清
支原体祛除试剂
干细胞培养基
- 细胞培养进口血清进口胎牛血清进口新生牛血清进口猪血清马血清
- 支原体检测盒及标准品常规PCR检测试剂盒荧光定量PCR检测(qPCR法)支原体DNA提取灵敏度标准品(方法验证用)特异性标准品(方法验证用)PCR定量标准品(可用于方法验证)
- 支原体祛除试剂细胞中支原体祛除环境支原体祛除水槽支原体祛除
- 干细胞培养基
- DNA/RNA污染祛除DNA/RNA污染祛除试剂DNA污染监测
- RNA病毒研究试剂RNA病毒检测试剂盒病毒RNA提取
- PCR仪器及配套产品DNA污染监测祛除PCR/qPCR仪性能检查PCR试剂PCR试剂盒PCR预混液(冻干粉)热启动聚合酶MB Taq DNA
- 微生物PCR检测食品检测类产品食品微生物检测细菌PCR检测
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在马铃薯试管薯使用临时浸没在液体培养基中2016-11-30 10:11
developed a new apparatus for plant tissue culture, using temporary immersion in a liquid medium. This apparatus was adapted to the microtuber production in potato. The procedure is as follows: single node cultivation on MS medium containing 30 g/l sucrose in the light for 2 weeks, induction of microtuberisation with 80 g/l sucrose over a 2 week period in the light, followed by a further 6 weeks in the dark. All experiments were performed at 20 °C. The basic vessel had a capacity of approximately 11;30 nodes were cultivated per vessel. Depending on the cultivars tested 47 to 115 microtubers were harvested per vessel. Between 30 and 60% of the microtubers weighted over 0.5 g and between 10 and 40% over 0.8 g. Sprouting is still under investigation. Preliminary results indicate that the dormancy period was relatively short and several stems were obtained per microtuber. These results seem to be better than those usually reported. Only one simple protocol has been tested and further improvements are probably easy to obtain. 版权声明:版权归原作者所有,如有版权问题,请与我们联系。
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