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Efficient genetic transformation of Jatropha curcas L. by microprojectile bombardment using embryo axes.

机译:利用胚轴轰击小麻疯树的有效遗传转化。

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An efficient and reproducible protocol was established for genetic transformation in Jatropha curcas through microprojectile bombardment. Decotyledonated embryos from mature seeds were pre-cultured for 5 days and elongated embryonic axis was subjected to bombardment for the optimization of physical parameters. The frequency of transient gus expression and survival of putative transformants were taken into consideration for the assessment of physical parameters. Statistical analysis reveal that microcarrier size, helium pressure and target distance had significant influence on transformation efficiency. Among different variables evaluated, microcarrier size 1 micro m, He pressure 1100 and 1350 psi with a target distance of 9 and 12 cm respectively were found optimum by co-relating microcarrier size, helium pressure and target distance on the frequency of gus expression and survival of putative transformants. Selection of putative transformants was done with increasing concentrations (5-7 mg L-1) of hygromycin. The integration of desired gene into Jatropha genome was confirmed with PCR amplification of 0.96 and 1.28 kb bands of hptII and gus gene respectively from the T0 transgenics and Southern blot analysis using PCR amplified DIG labeled hptII gene as a probe. A successful attempt of genetic transformation was made with optimized conditions using particle gene gun and establishing a stable transformation in J. curcas with 44.7% transformation efficiency. The procedure described will be very useful for the introgression of desired genes into J. curcas and the molecular analysis of gene function.
机译:通过微粒轰击建立了麻疯树的遗传转化的有效且可重复的方案。将来自成熟种子的去十子叶化胚进行预培养5天,并对细长的胚轴进行轰击以优化物理参数。瞬时 gus 的表达频率和推定的转化子的存活率被用于评估物理参数。统计分析表明,微载体的大小,氦气压力和靶距对转化效率有显着影响。通过将微载体尺寸,氦气压力和目标距离与gus频率相关联,可以发现在评估的不同变量中,微载体尺寸1 microm,He压力1100和1350 psi(目标距离分别为9和12 cm)是最佳的推定转化子的表达和存活。通过增加潮霉素浓度(5-7 mg L -1 )进行推定的转化子的选择。 PCR扩增了 hptII 和 gus 基因的0.96和1.28 kb条带,证实了所需基因已整合到 Jatropha 基因组中PCR扩增的DIG标记的 hptII 基因为探针,对> T 0 转基因和Southern印迹分析。使用粒子基因枪在最佳条件下成功进行了遗传转化,并在J中建立了稳定的转化。 curcas ,转化效率为44.7%。所描述的程序对于将所需基因渗入J非常有用。 curcas 和基因功能的分子分析。

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