利用回交法与Wx基因分子标记辅助选择培育糯性小麦

以中国春糯性位点全套近等基因系为研究材料,对小麦Wx基因的6个STS标记和1个CAPS标记进行了筛选。改良PCR扩增条件以及产物检测方式后,从这些标记中筛选出3个标记,包括鉴定Wx-A1、Wx-D1位点的2个共显性STS标记和Wx-B1位点的1个显性STS标记,用于本研究中糯性小麦的分子标记辅助育种。在育种过程中,首先配制全糯材料“98Y1441”与推广品种“川育12”的杂交组合,采用籽粒碘染法从其F2种子中选择全糯基因型个体与回交亲本川育12杂交,如此反复自交、回交,历经数代异地加代繁殖得到BC5F2代回交改良群体。利用上述3个分子标记从该群体中筛选出了8种Wx基因型,经卡方检验,其分离比符合3对基因的分离比例,其中基因型为aabbdd的植株有2株,直链淀粉含量分别为1.81%和0.82%,为全糯小麦;基因型为AAbbdd, aabbDD的部分糯性植株各有1株,直链淀粉含量分别为15.24%和17.57%。研究中获得的BC5 F2代群体的农艺性状接近回交亲本,并明显优于全糯材料“98Y1441”,表明采用回交法与Wx基因分子标记辅助选择相结合,有助于培育高产、优质的全糯和部分糯小麦。     

青海糯性春小麦综合标记辅助育种研究

选用全糯小麦品种‘糯麦1号’与青海主要栽培品种‘阿勃’杂交,综合利用改良碘染色法、SDS-PAGE法和Waxy基因的分子标记等,对杂交后代进行了鉴定筛选。最终从F2代鉴定出了5粒全糯种子,从F3代鉴定出8株Wx-B1亚基缺失的植株。对全糯株系F3代的农艺性状进行评价,5个全糯株系的综合农艺性状都优于‘糯麦1号’,与‘阿勃’较接近。测定全糯株系和Wx-B1亚基缺失植株F4代种子的直链淀粉含量,5个全糯株系F4代种子的直链淀粉含量接近于0,8个Wx-B1亚基缺失植株F4代种子的直链淀粉含量在总体上比‘阿勃’的直链淀粉含量低。研究表明,采用综合标记辅助选择可快速而准确地获得适合在青海栽培的全糯和部分糯性小麦。     

利用wx基因分子标记辅助选择培育糯性小麦

利用中国春及其缺体-四体对wx-B1基因的STS标记和wx-A1、wx-D1的微卫星(SSR)标记进行了定位.联合应用这2种分子标记,对12个小麦品种和5个高代糯麦株系做了鉴定,与Wx蛋白的SDS-PAGE结果一致;从组合江苏白火麦×关东107的F2分离群体中筛选出8种wx基因型,其中3种基因型(AD同缺型,BD同缺型和糯型)为自然界中所没有,并且培育出了国内首批糯性小麦品系.另外,应用SSR标记对江苏白火麦回交改良群体中个体进行辅助选择,得到了含wx-D1b的7D单体,为将来进一步改良糯性小麦的农艺性状提供广泛的遗传材料.利用wx基因分子标记辅助选择,可以加速培育糯性小麦的进程.     

多种优质高分子量谷蛋白亚基的聚合育种研究

用携带HMW-GS14 15的小偃6号作为轮回亲本,携带HMW-GS5 10的法国优质面包小麦品系707作为供体亲本,在回交后代的BC1、BC2、BC3、BC3F1、BC3F2代其它农艺性状选择的基础上,利用1对特异引物逐代检测出携带优质,Dx5基因的单株进行回交和自交。BC1代中随机检测的58个单株的Dx5基因分布符合1对等位基因的遗传分离比例1：1;BC1代小麦相同3个单株3个不同生长季节Dx5基因检测的结果完全一致,检测结果非常稳定;已将优质Dx5基因导入BC3F2后代的部分单株内;携带Dx5基因的株系XN89-7-3微量SDS沉淀值为18．8mL,比小偃6号提高了23．68％;蛋白质电泳筛选出了6个聚合多种优质亚基且编码基因纯合的单株,微量SDS沉淀值为19．9mL,比小偃6号提高了30．92％;选择农艺性状与轮回亲本相似并具有Dx5基因特异扩增产物的单株进行回交或自交,可加快回交转育的进度。实践证明,回交转育与分子标记辅助选育相结合的育种方法是快速定向聚合多种优质HMW-GS基因的有效方法之一。     

47份外引小麦种质资源Waxy和HMW-GS分子检测与品质性状分析

为有效利用外引小麦种质资源,本研究对收集的47份外引小麦种质材料进行Waxy和HMW-GS等位基因的分子检测,并分析了其直链淀粉、支链淀粉、湿面筋等品质参数。结果表明,在Wx-A1位点存在3种类型:Wx-A1a、Wx-A1g和WxA1b,39份材料(82.98%)为Wx-A1a类型;Wx-B1位点3种类型:Wx-B1a、Wx-B1e和Wx-B1b,37份材料(78.72%)为Wx-B1a类型;Wx-D1位点2种类型:Wx-D1a和Wx-D1b,46份材料具有Wx-D1a类型;共鉴定出8种Wx-1位点等位基因组合,31份材料(65.96%)为Wx-A1a/B1a/D1a。在Glu-A1位点,含有等位基因Ax2^*、Null和Ax1类型的材料分别为18份、18份和11份;在Glu-D1位点,含有等位基因Dx2和Dx5类型的材料分别为23份(48.94%)和21份(44.68%),含有等位基因Dy12和Dy10类型的材料分别为22份(46.81%)和20份(42.55%),具有Dy10+Dy12类型材料2份;共鉴定出19种Glu-A1/D1等位基因组合,7份材料含有Null/Dx5+Dy12。含有Wx-A1a/B1a/D1a材料的直链淀粉含量相对较高,支链淀粉含量相对较低;含有优质等位基因Ax1或Ax2^*兼Dx5+Dy10材料的湿面筋含量相对较高。总体上这些外引种质资源Waxy和HMW-GS等位基因类型丰富,可为种质资源合理利用和现代普通小麦品质改良提供参考依据。     

一种桔小实蝇蛹白化突变体的遗传分析

在实验室饲养野生型桔小实蝇Bactrocera dorsalis(Hendel)过程中发现了一种蛹色为白色的桔小实蝇突变品系。根据孟德尔遗传规律,设计野生型与突变型杂交(正交和反交)、F_1代与突变型回交、F_1代自交以及F_2代突变型自交等实验,对蛹白化突变性状的遗传规律进行研究。结果显示野生型与突变型杂交F_1代蛹色全部为野生型;F_2代野生型和突变型的性状分离比为2.98∶1,回交实验野生型与突变型性状分离比为1.19∶1;而突变体自交后代(F_3代)全部为突变体。结果表明桔小实蝇蛹色白化突变品系的遗传规律符合孟德尔遗传规律,属于常染色体上单基因控制的隐性遗传性状。     

定向改良超级早稻中早39稻瘟病抗性

稻瘟病是水稻生产中最具毁灭性的病害之一,稻瘟病菌生理小种变异快,抗性品种推广3～5年后抗性衰退风险较高,改良及培育抗稻瘟病菌新致病小种的品种是防治该病害最经济有效的方法。本研究以携带稻瘟病抗性基因Pi25的材料R6为供体亲本,超级早稻中早39为受体亲本和轮回亲本,通过杂交、回交和自交以及分子标记辅助选择技术,并结合室内喷雾接种、田间注射接种叶瘟以及病圃自然发病区穗颈瘟鉴定。综合考量抗性表型、基因型以及农艺性状,筛选出4个携带Pi25基因,叶瘟及穗颈瘟抗性较中早39提高,且农艺性状良好的株系FY82、FY90、FY125、FY137,同时对育成品系的系谱组成和抗性相关位点进行研究,初步阐明了育成品系较轮回亲本抗性水平提高的遗传基础。     

大豆蛋白质含量的遗传变异及其与主要农艺性状的相关性分析

摘要：以综合性状优良的黄淮海区主栽大豆品种中黄13为轮回亲本,从大豆微核心种质中选择蛋白质含量显著低于或高于轮回亲本的中黄20、东山69、迟黄豆-1和泰兴牛毛黄乙等4个品种作为供体亲本,比较分析了4个组合的RP、DP、F2、BC1F2和BC2F2蛋白质含量的遗传变异及其与主要农艺性状的相关性,结果表明,双亲蛋白质含量高有利于提高其杂交、回交后代的蛋白质平均含量及超轮回亲本个体比例;F2、BC1F2和BC2F2群体蛋白质含量的变异系数依次降低,BC2F2的蛋白质平均含量及其变异系数接近于轮回亲本;蛋白质含量在F2群体内呈正态分布,在双亲蛋白质含量高的组合中,其BC1F2群体呈偏态分布,但在BC2F2群体恢复了正态分布,稳定较快;供体亲本与其杂交2代、回交1代和回交2代在蛋白质含量、脂肪含量、株高、单株荚数、单株粒数、百粒重等性状上呈显著或极显著相关。     

CRISPR/Cas9介导基因组编辑培育糯稻不育系WX209A

糯稻作为特种稻米每年在我国和广西都有一定比例的消费,为了培育高产糯稻品种,本研究利用CRISPR/Cas9介导基因组编辑技术将高产的非糯性品种转为糯性品种,对水稻优良保持系209B中的W_x位点进行定点编辑,并转育成糯稻不育系WX209A。209A又名银丰A,是优良籼稻不育系,已组配出一批水稻品种在广西、广东、江西等地进行大面积推广。本研究针对该保持系的Wx基因选择合适的靶位点,构建sgRNA表达盒与 YLCRISPR/Cas9载体连接,利用农杆菌介导转化209B;对T_0、T_1代转化植株定点编辑位置进行PCR检测和测序分析及测定转化植株精米直链淀粉含量,筛选出无外源转化原件的纯合保持系WX209B并转育出不育系WX209A。结果表明,T_0代材料中Wx位点的突变频率高达69.2%,其中纯合缺失突变率占26.9%;对T_1代纯合突变体的调查分析结果表明,多数W_x基因突变体能显著降低直链淀粉含量,所获得的糯稻保持系WX209B直链淀粉含量仅1%,糯性品质优良,其他形态、经济性状没发生显著的改变,所转育的糯稻不育系WX209A具有重要的利用价值。     

一个新的小麦黄化突变体的遗传研究

摘要: 通过对冬小麦“西农1718” 自然黄化突变体多年连续自交、与突变亲本回交以及与其他基因型进行正反交, 研究突变性状的遗传规律。观察统计发现, 突变体中金黄株发育至抽穗－开花期前后死亡, 黄-绿株自交后代表现为1金黄株︰2黄-绿株︰1绿株, 绿株自交后代不再分离; 黄-绿株与突变亲本回交及与其他基因型正反交, 后代均表现为1黄-绿株︰1绿株。遗传分析表明, 该小麦黄化突变体是由一对核基因控制的不完全显性遗传, 其中, 金黄株是纯合体(au/au), 表现为致死, 黄-绿株为杂合体(Au/au), 绿株为纯合体(Au/Au)。     

Detection of single nucleotide polymorphism (SNP) controlling the waxy character in wheat by using a derived cleaved amplified polymorphic sequence (dCAPS) marker

We investigated a single nucleotide polymorphism (SNP) in the Wx-D1 gene, which was found in a mutant waxy wheat, and which expressed the Wx-D1 protein (granule-bound starch synthase I) as shown by immunoblot analysis. We also assayed starch synthase activity of granule-bound proteins. Using 22 doubled-haploid (DH) lines and 172 F(5) lines derived from the wild type x the mutant, we detected SNP via a PCR-based (dCAPS) marker. Amplified PCR products from Wx-D1 gene-specific primers, followed by mismatched primers designed for dCAPS analysis, were digested with the appropriate restriction enzyme. The two alleles, and the heterozygote genotype were easily and rapidly discriminated by gel-electrophoresis resolution to reveal SNP. All progeny lines that have the SNP of the mutant allele were waxy. Integrating the results of dCAPS analysis, immunoblot analysis and assays of starch synthase activity of granule-bound proteins indicates that the SNP in the Wx-D1 gene was responsible for its waxy character. This dCAPS marker is therefore useful as a marker to introduce the mutant allele into elite breeding lines.     

Rapid classification of partial waxy wheats using PCR-based markers.

Mutations in the three homeologous waxy loci Wx-A1, Wx-B1, and Wx-D1 of a waxy wheat line have previously been characterized at the molecular level. Using combinations of these mutations, six types of partial waxy wheat plus wild type and waxy wheat (types 1-8) can be produced. Here, we describe primer sets for all three loci that can be used under a single set of conditions, allowing 32 lines to be characterized as types 1-8 in a single PCR run using a 96-well plate. Using multiplex PCR, mutations at the Wx-B1 and Wx-D1 loci can be identified in a single PCR, reducing the number of reactions necessary to identify and select the desired partial waxy wheat line. A single multiplex PCR can be used to detect all three mutations when products are analyzed using capillary electrophoresis on a microchip device. The PCR conditions and primers are effective with a number of cultivars from other countries, indicating that the mutations found at the Wx-A1 and Wx-B1 loci of these cultivars likely have the same origins as the mutations in the corresponding loci of the waxy wheat line used in this study. The PCR selection method described here is an easy and effective alternative to the commonly used SDS-PAGE methods for identification of null alleles.     

A novel codominant marker for selection of the null Wx-B1 allele in wheat breeding programs

Waxy protein (granule-bound starch synthase I) is a key enzyme in the synthesis of amylose in endosperm tissue. The amylose content of wheat flour plays a significant role in determining Japanese udon noodle quality. Most wheat cultivars suitable for producing udon noodles have a low amylose level due to a lack of Wx-B1 protein conditioned by null Wx-B1 alleles. It was previously determined that the entire coding region of the wheat Wx-B1 gene is deleted in the most common null allele. However, the extent and breakpoints of the deletion have not been established. In this study, the position of the 3′ deletion breakpoint was refined by mapping with PCR-based markers. Using information from this analysis, a chromosome walk was initiated and the DNA sequence flanking the deletion breakpoints was obtained. The deletion included a 3,872 bp region downstream from the termination codon of Wx-B1 gene. Based on similarity with T. monococcum sequences, it was estimated that approximately 60 kb upstream of the Wx-B1 gene was also deleted. Using this sequence information, a codominant marker for the identification of the Wx-B1 null allele was developed. This marker can unambiguously identify heterozygous plants, which will accelerate the selection of partial waxy mutants carrying the Wx-B1 null allele.     

Waxy protein deficiency and chromosomal location of coding genes in common wheat

Deficiency of the wheat waxy (Wx) proteins (Wx-A1, Wx-B1 and Wx-D1) was studied in 1,960 cultivars derived from several countries. Gel electrophoretic analyses revealed that the null allele for the Wx-A1 protein occurred frequently in Korean, Japanese and Turkish wheats but was relatively rare in cultivars from other countries and regions. About 48% of the wheats deficient for the Wx-B1 protein were from Australia and India. One Chinese cultivar lacked the WxD1 protein. While 9 Japanese cultivars were deficient in both the Wx-A1 and Wx-B1 proteins, no cultivars lacked both the Wx-A1 and Wx-D1 proteins, both the Wx-B1 and Wx-D1 proteins or all three Wx proteins. Two-dimensional gel electrophoresis revealed polymorphisms of the three Wx proteins that varied according to isoelectric points or molecular weight. The Wx-A1 gene coding the Wx-A1 protein and the Wx-B1 gene coding the Wx-B1 protein were localized in the distal regions of chromosome arms 7AS and 4AL, respectively, by deletion mapping using the deletion lines developed in the common wheat cultivar Chinese Spring.     

籼稻花粉无性系变异的研究

对７个籼稻品种通过花药培养获得的１６１个花粉植株进行了花粉无性系变异的研究。结果表明：（１）所有花粉无性系在遗传上都是纯合的,其整齐度与起始亲本相近或超过起始亲本;（２）花粉无性系的变异主要在数量性状上有一定变幅,变异方向有负向也有正向的。同一来源的无性系间的变异系数略高于起始亲本,仅千粒重达到显著标准。以所考查的性状为基数,变异的频率为１２．５％,同时有３－４个性状发生变异的无性系数占总数的４．３％;（３）少数变异体性状有重大变异,并具有育种价值;（４）根据１０种同工酶和ＲＦＬＰ分析,仅从３个性状发生重大变化的变异体中检测出与起始亲本的差异。     

基于MAS的小麦抗赤霉病育种材料抗性评价

为了提高黄淮海麦区小麦育种材料的赤霉病抗性,采用分子标记辅助选择的方法,将来自望水白的4个抗赤霉病主效QTL 3B-QTL、4B-QTL、5A-QTL和6B-QTL导入不同的感病背景中,在后代BC1F3和BC1F4株系中评价它们的抗病效应和农艺性状回复情况。结果表明:(1)导入4个抗病QTL株系的平均病小穗率和病粒率分别为12.2%和6.3%,而受体亲本则分别达到59.1%和44.2%,抗病性显著提高;(2)病小穗数和病粒率与穗长及株高极显著负相关,但与可育小穗数、百粒重、旗叶长和旗叶宽等农艺性状指标没有显著相关性。因此,通过导入抗病主效QTL可以显著改善感病材料的抗性,为进一步选育高产抗病品种提供基础材料。不良农艺性状的紧密连锁阻碍着抗赤霉病主效QTL的高效利用,需要通过继续回交或与其他品种杂交来打破这种遗传连锁关系。