经基因工程改良的抗白叶枯病水稻粳型恢复系“C418-Xa21”及其杂交稻

通过农杆菌介导的转化系统,将业已克隆的水稻抗白叶枯病基因Xa21导入重要的粳型杂交稻恢复系“C418”。PCR和抗性分析表明单拷贝整合的Xa21在T₁代的分离比为3∶1。在T₂代通过PCR和抗性分析选择了Xa21纯合的转基因株系“C41-Xa21”。将选择的转基因纯合系“C418-Xa21”与常用的雄性不育系“屉锦A”杂交,产生了带有转基因Xa21的杂交稻“屉优41-Xa21”(简称转基因杂交稻)。分子分析表明转基因Xa21在杂交稻“屉优418-Xa21”中能稳定遗传;抗性分析表明转基因恢复系“C418-Xa21”和转基因杂交稻“屉优418-Xa21”对白叶枯病具有高度的广谱抗性,并保持了受体对照的优良农艺性状。另外我们还发现转基因杂交稻“屉优418-Xa21”对白叶枯病的抗性水平高于转基因恢复系“C418-Xa21”,这可能是遗传背景的差异所致。抗白叶枯病转基因粳型恢复系和杂交稻的育成将有益于杂交稻在我国北方稻区的推广。     

无选择标记和载体骨干序列的Xa21转基因水稻的获得

利用双右边界T-DNA载体通过根癌农杆菌介导法将水稻白叶枯病广谱抗性基因Xa21导入杂交稻重要恢复系C418中。T₀代共获得27个独立转基因株系,通过田间抗性鉴定与PCR分析,有17个株系的Xa21基因分子鉴定为阳性,且对白叶枯病原菌P6生理小种具有抗性。通过对17个株系的后代植株进行田间抗性鉴定,分子标记辅助选择及Southern杂交分析,结果显示4个株系的T₁代植株中能分离出无潮霉素标记基因的Xa21转基因植株。无选择标记Xa21转基因株系的获得率为15%。PCR检测还表明,这些无选择标记的Xa21转基因植株不带有载体骨架序列。通过对转基因后代进一步的抗性鉴定与PCR辅助选择,获得了无选择标记和载体骨架序列的转基因Xa21纯合的抗白叶枯病水稻。     

由农杆菌介导将白叶枯病抗性基因Xa21转入我国的5个水稻品种

利用农杆菌介导的转化系统将已克隆的Xa21基因转入我国5个水稻主栽品种, 获得了110个独立的转基因系. 转基因植株的PCR和Southern分析揭示Xa21基因已整合到受体基因组. 已整合的Xa21基因能稳定遗传, 单拷贝整合的转化体在自交T1代呈现抗感3:1的分离. 接种实验表明转基因T0植株和Xa21-PCR阳性T1植株对白叶枯病的高度抗性. 经过筛选的Xa21纯合的具有优良品质的抗性转基因系可以作为品种直接种植, 或者用于杂交稻育种.     

水稻白叶枯病广谱抗性基因Xa21导入两用不育系培矮64S

以克隆的Xa21基因为外源基因,成熟胚愈伤组织为转化受体,应用农杆菌介导法对水稻两用型核不育系培矮64S进行转化,获46株转基因植株。PCR和Southern分析结果表明,Xa21已整合到受体基因组。用稻白叶枯病病原菌(Xanthomonasoryzaepv.oryzae)菲律宾小种6号接种鉴定,结果表明大多数转基因植株获得了抗病性。已整合的Xa21基因能够稳定地遗传,在所检测转基因株系的T1代中,Xa21基因显示3:1的分离。     

水稻白叶枯病抗性基因Xa23鉴别菌株突变体库的构建及无毒基因突变体的筛选

利用invivo转座技术构建了白叶枯病抗性基因Xa23鉴别菌株的突变体库,特异性引物PCR扩增和转座子插入位点旁侧序列分析结果表明转座子插入到白叶枯病菌的基因组中。经人工接种鉴定,筛选到4个毒力发生变化的突变体。为进一步克隆Xa23无毒基因提供了条件。     

菜豆重金属响应基因PvSR2在烟草中的表达及镉抗性分析

重金属特异诱导基因PvSR2(Phaseolus vulgaris stress-related)是从法国菜豆中克隆出来的, 为了研究该蛋白能否提高植物的抗重金属能力, 将PvSR2基因插入到植物转化中间载体pCAMBIA2301中CaMV 35S启动子的下游, 用根癌农杆菌介导的叶盘法将其导入烟草中, 在含有100 mg/L Kan的MS培养基上筛选, 获得了转基因植株. PCR和Southern杂交结果表明PvSR2已整合在烟草基因组中, GUS和Northern分析表明PvSR2在转基因烟草中获得表达. 重金属抗性实验表明: 与野生型烟草相比, PvSR2转基因烟草具有较高的抗重金属镉(Cd)的能力. 组织Cd含量分析显示: 在低浓度Cd (0.5~0.75 mmol/L)处理时, Cd在PvSR2转基因烟草与野生型烟草根中的累积量没有明显的差别, 而在高浓度Cd(0.1 mmol/L)胁迫下, 转基因烟草根中Cd的累积量低于野生型烟草, 说明PvSR2的表达能够提高植物的抗重金属能力, 同时表明PvSR2可能与重金属在植物中的运输和积累有一定关系.     

转修饰cry1Ac基因籼稻明恢81经花药培养获得抗虫DH系

对基因枪法获得的明恢81转修饰的cry1Ac基因当代植株进行花药培养,共接种花药2600枚,获得83份花培植株,其中双倍体植株43份,单倍体植株40份。 PCR结果表明含有cry1Ac基因的植株55份,花培植株群体中转基因与非转基因植株的比值为2∶1（55/28）。进一步结合Southern blot和ELISA分析,于花培植株当代筛选到转基因纯合株系36份。外源蛋白表达量上,花药来源于同一克隆的DH系的不同植株之间基本一致,最高的Cry1Ac含量达0.25%。田间抗虫性试验表明,经花药培养纯合获得的部分转基因纯合系植株对二化螟(Chilo suppressalis)表现出高抗,而且主要农艺性状保持不变。以上结果表明水稻花药培养可以加速转基因的纯合与育种利用。     

转Xa21基因水稻中T-DNA整合的遗传定位

利用转抗白叶枯病基因Xa21的水稻材料,通过TAIL－PCR方法扩增T－DNA整合的侧翼序列。从中筛选属于水稻基因组DNA的T－DNA整合的侧翼序列作为探针,将外源基因整合位点定位到窄叶青／京系17DH群体构建的水稻分子连锁图谱上。共获得属于水稻基因组DNA的T－DNA侧翼序列22个,其中的19个序列在定位群体的两个亲本之间显示RFLP多态性,分别定位在水稻基因组的第3,4,5,7,9,10,11和12染色体上。带有转基因Xa21的T－DNA整合的定位为研究外源基因在不同染色体位点的位置效应和稳定遗传打下基础。     

TAIL-PCR方法快速分离Xcc致病相关基因序列

以miniTn5gfp-km转座子中nptII片段作为探针,对已获得的五株野油菜黄单胞菌野油菜黑腐病致病型（Xcc）非致病突变体进行了Southern blot分析,结果表明,这五株突变体确由mini-Tn5gfp-km转座子插入致病相关基因所致,且为单拷贝不同位点的插入。提取这五株突变体总DNA作为模板,采用改进的热不对称交错PCR （TAIL-PCR）方法从其中克隆到了各自转座子插入区侧翼序列,对这些侧翼序列进行了序列测定并将分析结果与GenBank database及Xcc全基因组序列做了比较,结果表明,五个侧翼序列所在的基因确与Xcc致病性有关。这种改进后的TAIL-PCR方法为突变体特别是转座子插入突变体中目的基因的克隆提供了一种简便高效的新方法。     

转基因水稻中转录水平cry1Ab 基因的沉默及其阶段复活

以田间环境释放条件下农杆菌介导法转化而成的转cry1Ab 基因水稻为研究对象, 利用GUS组织化学染色法、Western杂交技术, 在不抗虫转基因中8215株系后代中筛选到一个无cry1Ab 蛋白表达产物株系. 分子杂交结果证实, 转基因cry1Ab 在中8215株系后代中发生了转录水平沉默, 整合过程中基因重排使两个拷贝的ubiquitin启动子同时插入到水稻基因组中. 甲基化分析证实ubiquitin启动子区域发生了甲基化, 从而导致cry1Ab基因沉默. 利用去甲基化试剂5-氮胞苷处理转基因沉默水稻种子, 并在苗期、分蘖期、孕穗期、灌浆期及成熟期检测了其对沉默基因的复活效应, 结果表明：5-氮胞苷处理使沉默的cry1Ab 基因在灌浆期恢复表达活性, 复活率约为8%~30%, 且以低浓度(45 mg/L处理1, 2 d)处理的复活率及恢复表达水平较高, 复活基因表达的cry1Ab 蛋白最高可达可溶性总蛋白的0.147%.     

Analysis of T-DNA-<Emphasis Type="Italic">Xa21</Emphasis> loci and bacterial blight resistance effects of the transgene <Emphasis Type="Italic">Xa21</Emphasis> in transgenic rice

The genetic loci and phenotypic effects of the transgene Xa21, a bacterial blight (BB) resistance gene cloned from rice, were investigated in transgenic rice produced through an Agrobacterium-mediated transformation system. The flanking sequences of integrated T-DNAs were isolated from Xa21 transgenic rice lines using thermal asymmetric interlaced PCR. Based on the analysis of 24 T-DNA- Xa21 flanking sequences, T-DNA loci in rice could be classified into three types: the typical T-DNA integration with the definite left and right borders, the T-DNA integration linked with the adjacent vector backbone sequences and the T-DNA integration involved in a complicated recombination in the flanking sequences. The T-DNA integration in rice was similar to that in dicotyledonous genomes but was significantly different from the integration produced through direct DNA transformation approaches. All three types of integrated transgene Xa21 could be stably inherited and expressed the BB resistance through derived generations in their respective transgenic lines. The flanking sequences of the typical T-DNA integration consisted of actual rice genomic DNA and could be used as probes to locate the transgene on the rice genetic map. A total of 15 different rice T-DNA flanking sequences were identified. They displayed restriction fragment length polymorphisms (RFLPs) between two rice varieties, ZYQ8 and JX17, and were mapped on rice chromosomes 1, 3, 4, 5, 7, 9, 10, 11 and 12, respectively, by using a double haploid population derived from a cross between ZYQ8 and JX17. The blast search and homology comparison of the rice T-DNA flanking sequences with the rice chromosome-anchored sequence database confirmed the RFLP mapping results. On the basis of genetic mapping of the T-DNA- Xa21 loci, the BB resistance effects of the transgene Xa21 at different chromosome locations were investigated using homozygous transgenic lines with only one copy of the transgene. Among the transgenic lines, no obvious position effects of the transgene Xa21 were observed. In addition, the BB resistance levels of the Xa21 transgenic plants with different transgene copy numbers and on different genetic backgrounds were also investigated. It was observed that genetic background (or genome) effects were more obvious than dosage effects and position effects on the BB resistance level of the transgenic plants.     

经基因工程改良的抗白叶枯病水稻粳型恢复系“C418—Xa21”及其杂交稻

通过农杆菌介导的转化系统,将业已克隆的水稻抗白叶枯病基因Xa21导入重要的粳型杂交稻恢复系“C418”。PCR和抗性分析表明单拷贝整合的Xa21在T1代的分离比为3：1。在T2代通过PCR和抗性分析选择了Xa21纯合的转基因株系“C418－Xa21”。将选择的转基因纯合系“C418－Xa21”与常用的雄性不育系“屉锦A”杂交,产生了带有转基因Xa21的杂交稻“屉优418－Xa21”（简称转基因杂交稻）。分子分析表明转基因Xa21在杂交稻“屉优418－Xa21”中能稳定遗传,抗性分析表明转基因恢复系“C418－Xa21”和转基因杂交稻“屉优418－Xa21”对白叶枯病具有高度的广谱抗性,并保持了受体对照的优良农艺性状。另外我们还转基因杂交稻“屉优418－Xa21”对白叶枯病的抗性水平高于转基因恢复系“C418－Xa21”,这可能是遗传背景的差异所致,抗白叶枯病转基因粳型恢复系数 杂交稻的育成将有益于杂交稻在我国北方稻区的推广。     

水稻转基因系"明恢63-Xa21"的基因组分析

植物基因工程研究已经建立了多种转基因的方法 ,这些方法包括农杆菌侵染[1 ] 、粒子轰击[2 ] 、电激转化和原生质体培养[3 ] 等。研究人员希望通过这些方法 ,将功能外源基因整合到受体基因组 ,而同时不引起其它性状的变化。已有的研究表明 ,各种转基因系统均能成功地将外源基因整合到受体基因组并能稳定地遗传到后代[1～ 3 ] 。然而通常情况下人们主要关注目标性状的变化 ,而对受体基因组的其它变化研究较少。事实上许多转基因植物发生了不希望出现的变异[4,5] 。已建立的各种分子标记如ＳＳＲＰ(简单序列重复多态性 ) [6] 、ＲＡＰＤ(随机…     

Breeding bacterial blight-resistant hybrid rice with the cloned bacterial blight resistance gene Xa21

The cloned bacterial blight (BB) resistance gene Xa21 was transferred into Minghui63, a widely used restorer line of indica hybrid rice in China, through an Agrobacterium-mediated system. Molecular and resistance analyses revealed that the Xa21 gene was integrated in the genomes of transgenic plants and their progeny inherited resistance stably. For the purpose of hybrid breeding, Xa21 transgenic homozygous restorer lines were selected through `within-lane' dosage comparison of hybridization signal in combination with PCR and resistance analyses. The selected transgenic restorer lines were then crossed with a commonly used sterile line, Zhenshan97A, to produce Xa21 transgenic hybrid rice, Shanyou63-Xa21. The hybrid rice plants with Xa21 displayed high broad-spectrum resistance to Xanthomonas oryzae pv. oryzae (Xoo) races and maintained elite agronomic characters of Shanyou63. The propagation of this BB-resistant hybrid variety with Xa21 will benefit rice production.     

Introduction of a rice blight resistance gene,Xa21, into five Chinese rice varieties through anAgrobacterium-mediated system

A cloned gene, Xa21 was transferred into five widely-used Chinese rice varieties through an Agrobacterium-mediated system, and over 110 independent transgenic lines were obtained. PCR and Southern analysis of transgenic plants revealed the integration of the whole Xa21 gene into the host genomes. The integrated Xa21 gene was stably inherited, and segregated in a 3 : 1 ratio in the selfed T1 generation when one copy of the gene was integrated in the transfor-mants. Inoculation tests displayed that transgenic T0 plants and Xa21 PCR-positive T1 plants were highly resistant to bacterial blight disease. The selected Xa21 homozygous resistant transgenic lines with desirable qualities may be propagated as new varieties or utilized in hybrid rice breeding.     

Introduction of a rice blight resistance gene, Xa21, into five Chinese rice varieties through an Agrobacterium-mediated system

A cloned gene, Xa21 was transferred into five widely-used Chinese rice varieties through an Agrobacterium-mediated system, and over 110 independent transgenic lines were obtained. PCR and Southern analysis of transgenic plants revealed the integration of the whole Xa21 gene into the host genomes. The integrated Xa21 gene was stably inherited, and segregated in a 3∶1 ratio in the selfed T1 generation when one copy of the gene was integrated in the transformants. Inoculation tests displayed that transgenic T0 plants and Xa21 PCR-positive T1 plants were highly resistant to bacterial blight disease. The selected Xa21 homozygous resistant transgenic lines with desirable qualities may be propagated as new varieties or utilized in hybrid rice breeding.     

Xa26, a gene conferring resistance to Xanthomonas oryzae pv. oryzae in rice, encodes an LRR receptor kinase-like protein

Rice bacterial blight, caused by Xanthomonas oryzae pv. oryzae (Xoo), is one of the most serious rice diseases worldwide. A rice gene, Xa26, conferring resistance against Xoo at both seedling and adult stages was isolated by map-based cloning strategies from the rice cultivar Minghui 63. Xa26 belongs to a multigene family consisting of four members. It encodes a leucine-rich repeat (LRR) receptor kinase-like protein and is constitutively expressed. Sequence analysis revealed that IRBB3 and Zhachanglong lines that are resistant to a broad range of Xoo strains, also carry Xa26. However, significant difference in lesion length was observed among these lines after inoculation with a set of Xoo strains. Moreover, transgenic plants carrying Xa26 showed enhanced resistance compared with the donor line of the gene in both seedling and adult stages. These results suggest that the resistance conferred by Xa26 is influenced by the genetic background.     

Pyramiding transgenic resistance in elite indica rice cultivars against the sheath blight and bacterial blight

Elite indica rice cultivars were cotransformed with genes expressing a rice chitinase (chi11) and a thaumatin-like protein (tlp) conferring resistance to fungal pathogens and a serine-threonine kinase (Xa21) conferring bacterial blight resistance, through particle bombardment, with a view to pyramiding sheath blight and bacterial blight resistance. Molecular analyses of putative transgenic lines by polymerase chain reaction, Southern Blot hybridization, and Western Blotting revealed stable integration and expression of the transgenes in a few independent transgenic lines. Progeny analyses showed the stable inheritance of transgenes to their progeny. Coexpression of chitinase and thaumatin-like protein in the progenies of a transgenic Pusa Basmati1 line revealed an enhanced resistance to the sheath blight pathogen, Rhizoctonia solani, as compared to that in the lines expressing the individual genes. A transgenic Pusa Basmati1 line pyramided with chi11, tlp, and Xa21 showed an enhanced resistance to both sheath blight and bacterial blight. S. Maruthasalam and K. Kalpana have contributed to this article equally.