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番茄品种叶片叶肉原生质体的再生:影响原生质体高效培养和植株再生的重要因素。

Regeneration of leaf mesophyll protoplasts of tomato cultivars (L. esculentum): factors important for efficient protoplast culture and plant regeneration.

机构信息

Department of Genetics, Free University, De Boelelaan 1087, 1081 HV, Amsterdam, The Netherlands.

出版信息

Plant Cell Rep. 1987 Jun;6(3):172-5. doi: 10.1007/BF00268470.

Abstract

Conditions were established for efficient plant regeneration from four freshmarket cultivars of Lycopersicon esculentum. In order to increase the yield of viable protoplasts which are able to sustain cell divisions, the donor plants are preconditioned by incubation at 25°C in the dark for 18 hours, followed by a cold treatment at 4°C in the dark for the last 6 hours, prior to protoplast isolation. Browning of the dividing cell colonies can be prevented by culturing protoplasts in 100 μl droplets of low-melting agarose, surrounded by liquid medium. Alternatively, protoplasts can be cultured in liquid medium. In both procedures the plating efficiencies and percentage of shoot regeneration are increased, only when dilutions were performed with auxin-free culture medium. Shoot regeneration is obtained by using a two step procedure: initiation of greening of microcalli on a medium containing 0.2 M mannitol and 7.3 mM sucrose, which is followed by shoot development on a mannitol-free medium containing 0.5 M sucrose. In this way, plants can be regenerated within 3 months from the hybrid cultivars Bellina, Abunda, Sonatine and also from the true seedline Moneymaker. The latter one showed the highest regeneration frequency (30%).

摘要

为了从四个新鲜市场品种的番茄中高效地进行植物再生,建立了条件。为了增加能够维持细胞分裂的有活力原生质体的产量,在原生质体分离之前,将供体植物在黑暗中于 25°C 下预培养 18 小时,然后在黑暗中于 4°C 下进行冷处理 6 小时。通过在低熔点琼脂糖的 100μl 液滴中培养原生质体,可以防止细胞分裂菌落的褐变,液滴周围是液体培养基。或者,原生质体可以在液体培养基中培养。在这两种程序中,只有在使用不含生长素的培养基进行稀释时,平板效率和芽再生率才会提高。通过两步程序获得芽再生:在含有 0.2M 甘露醇和 7.3mM 蔗糖的培养基上启动微愈伤组织的变绿,然后在不含甘露醇的培养基上(含有 0.5M 蔗糖)进行芽发育。通过这种方式,杂种品种 Bellina、Abunda、Sonatine 以及真正的种子系 Moneymaker 可以在 3 个月内再生植株。后者显示出最高的再生频率(30%)。

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