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苜蓿原生质体高效细胞分裂的诱导。

Induction of efficient cell division in alfalfa protoplasts.

机构信息

Ottawa Research Station, Agriculture Canada, K1A OC6, Ottawa, Canada.

出版信息

Plant Cell Rep. 1985 Oct;4(5):229-32. doi: 10.1007/BF00269364.

Abstract

Alfalfa (Medicago sativa L.) protoplasts derived from cell suspension cultures divided inefficiently in liquid culture. The onset of cell division activity occurred synchronously among the protoplasts; however, many were blocked at cytokinesis and therefore did not complete first division. Very few of the cells that began to divide continued to do so. Immobilization of protoplasts in agarose after 1 to 4 days in liquid culture overcame this inhibition of division. Continuous growth in agarose was restricted and therefore microcolonies were transferred to agar medium to complete callus development. Plating efficiencies of 2-10% were achieved within 30 days of protoplast isolation. The agarose treatment was responsible for a 5- to 30-fold improvement in plating efficiency.

摘要

苜蓿(Medicago sativa L.)原生质体由细胞悬浮培养物衍生而来,在液体培养中分裂效率低。细胞分裂活动的开始在原生质体中同步发生;然而,许多原生质体在胞质分裂时被阻断,因此无法完成第一次分裂。开始分裂的细胞中很少有继续分裂的。在液体培养 1 至 4 天后,将原生质体固定在琼脂糖中,可以克服这种分裂抑制。在琼脂糖中的连续生长受到限制,因此微菌落被转移到琼脂培养基中以完成愈伤组织的发育。在原生质体分离后的 30 天内,达到了 2-10%的平板效率。琼脂糖处理使平板效率提高了 5-30 倍。

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