中国白菜小孢子离体培养和双单倍体植株再生

采用略加修改的NLN培养基(无机大量元素1/2)和甘蓝型油菜小孢子的胚状体诱导程序,培养了5个中国菜用小白菜品种和1个中国大白菜品种的小孢子,进行了双单倍体的诱导。结果表明,不同品种的小孢子产胚量差异很大,在接种的6个基因型中,有5个诱导出胚,诱导率83.33%。其中的中萁青抗热605产胚量最高,是8.68个胚/10蕾,最低的是鸡冠菜,其产胚率是0.42个胚/10蕾。这些胚在添加了NAA和PP333(多效唑)的B5培养基发育成健壮的小植株,已移栽到田间。关于6个基因型的小孢子胚胎发生能力,还有待进一步研究。

利用离体小孢子培养技术培育心里美萝卜新品系

以北京心里美和山东心里美为供体材料进行离体小孢子培养,2个基因型均成功获得胚状体,每105个小孢子的成胚率分别为15.6%和21.3%。选取子叶形胚进行胚状体再生,北京心里美与山东心里美的成苗率分别为78.9%和64.5%。利用流式细胞仪对再生株倍性进行鉴定,44.8%为二倍体(双单倍体,DH系),17.2%为单倍体,38.1%为多倍体。选择正常的二倍体植株进行自交留种,并对自交后代进行田间性状鉴定,与供体植株相比,DH系出现较大的性状变异。对来源于北京心里美的肉质根圆形、绿皮血红肉和椭圆形、绿皮血红肉DH系进行扩繁,后代性状整齐一致,血红肉率100%,没有出现浅绿肉变异株。利用离体小孢子培养技术获得了肉色整齐一致的心里美萝卜新品系,有效解决了常规自交易出现浅绿肉变异株的问题。

小孢子和花药培养技术在作物定向遗传改良上的应用

介绍了小孢子/花药离体培养系统的特点以及应用于作物遗传改良的优点;回顾了研究室已有的单倍体细胞工程及育种的一些进展;对小孢子/花药离体培养系统在作物定向遗传改良应用的前景进行了探讨。

源于小孢子培养的大麦耐盐变异体获取

以大麦品种‘花30’作为供试材料,比较了甲基磺酸乙酯(EMS)和平阳霉素处理小孢子,60Coγ-射线辐照处理离体穗和干种子,对300mg·L-1NaCl胁迫培养下游离小孢子的愈伤组织产量和愈伤组织在0.3%NaCl胁迫筛选下的绿苗产量的影响。结果表明,EMS处理离体小孢子和60Coγ-射线辐照干种子的愈伤组织产量和绿苗产量明显优于平阳霉素处理小孢子和60Coγ-射线辐照离体穗。以16份源于种子辐照处理的再生植株自交一代种子为供试材料,比较了在0.3%NaCl胁迫下种子的发芽率和幼苗的成活率以及植株的分蘖数、株高和单株产量。结果表明,‘花30’发芽率为0,供试的16份耐盐变异体中,有14份材料在NaCl胁迫下的发芽率优于‘花30’,鉴定出4份耐盐性明显优于‘花30’的变异体材料。选择耐盐变异体作为供试材料,测定了变异体中Na+/H+逆向转运蛋白基因NHX1、NHX2和NHX3和编码甜菜碱醛脱氢酶(BADH)的两个同工酶基因BBD1和BBD2的表达模式和表达量,结果表明变异体耐盐性的提高与这些基因的表达量存在联系。

Establishment on Isolated Microspore Culture Optimized System for Restorer of New Cytoplasmic Male Sterile (NER) of Brassica napus L.

[Objective]The aim was to establish optimized system for NER isolated microspore culture of Brassica napus L.. [Method]Twenty varieties of NER of Brassica napus were grown under uncontrolled temperature and light conditions,and their isolated microspore from anthers were used as explants in vitro culture. The influencing factors of microspore culture were preliminarily studied. [Result]The difference of genotypes was important influencing factors to embryoid yield. The embryoid yield increased by supplementing with 6-BA and NAA,culturing in solid-liquid double layer medium with activated charcoal; The difference was not significant of embryoid yield between culturing in medium supplemented with colchicines and the CK. The rates of cotyledonous embryoids directly developed into normal plantlets increased through enriching with 0.1-0.2 mg/L NAA and being treated on slim illumination two days before being inducted into normal plantlets. [Conclusion]The technical system of microspore culture of restorer of new cytoplasmic male sterile （NER） was established,which and lays a foundation for accelerating genotype purification of NER introgressive line.