利用重组自交系群体定位玉米生育期相关性状QTL

利用玉米自交系80007和80044为亲本,衍生包含355个家系的重组自交系(RIL)F9群体,采用SSR标记构建包括219个标记的连锁图谱,图谱总长度2 133.5 cM,标记间平均距离9.7 cM。采用完备区间作图法对控制玉米抽雄期、散粉期、吐丝期以及散粉至吐丝间隔期的4个生育期相关性状进行QTL分析。结果表明,共检测到60个QTL,其中抽雄期检测到20个QTL,吐丝期检测到15个QTL,散粉期检测到20个QTL,散粉至吐丝间隔期检测到5个QTL。共有7个QTL对表型变异的解释率超过了10%,表现为主效QTL效应,分布在第3、4和第9染色体。有11个QTL在不同环境中能重复检测出,是受环境影响较小、为较稳定的QTL。分析发现,生育期相关性状的QTL在染色体上有"成簇"分布的现象,并且贡献率较大的QTL控制着多个相关性状。结果表明,bin3.04-3.05、bin3.09、bin7.03和bin9.02-9.03是生育期相关性状QTL的密集区域,这些区域存在对生育期相关性状重要作用的位点。     

四川小麦品种高、低分子量麦谷蛋白基因和1B/1R易位的分子标记鉴定

为给四川小麦品质育种提供参考信息,利用7个HMW-GS、17个LMW-GS和1个1B/1R易位的特异分子标记,对105份2000年后育成的四川小麦品种进行上述基因检测。结果表明:(1)针对HMWGS,在Glu-A1位点,含Ax2*的品种有2份,频率为1.9%;在Glu-B1位点,含Bx7、Bx20、Bx17、By8和By9的品种分别有73、26、4、45和30份,频率分别为69.5%、24.8%、3.8%、42.9%和28.6%,未检测到含Bx7OE的品种;在Glu-D1位点,含Dx5的品种有65份,频率为61.9%。(2)针对LMW-GS,在Glu-A3位点,含Glu-A3a、Glu-A3b、Glu-A3c、Glu-A3d和Glu-A3f的品种分别有2、2、63、29和9份,频率分别为1.9%、1.9%、60.0%、27.6%和8.6%,未检测到含Glu-A3e和Glu-A3g的品种;在Glu-B3位点,含Glu-B3b、Glu-B3d、Glu-B3f、GluB3g和Glu-B3i的品种分别有18、10、1、75和1份,频率分别为17.1%、9.5%、1.0%、71.4%和1.0%,未检测到含Glu-B3a、Glu-B3c、Glu-B3e和Glu-B3h的品种。(3)含1B/1R易位的品种有36份,频率为34.3%。(4)组合6种和5种以上优质基因的品种分别有2份(频率为3.8%)和15份(频率为14.3%)。可利用这些品种作为亲本,在四川小麦品质育种中逐步导入优质基因Ax2*、Bx7、By8、Dx5、Glu-A3d、Glu-B3d、Glu-A3b和Glu-B3b,并淘汰1B/1R易位,优化四川小麦面筋优质基因组成。     

小麦次生根数相关分子标记的挖掘

为了给小麦根系性状的遗传改良提供参考依据,以196份小麦自然群体为材料,于2013年拔节期和2014年越冬前、拔节期统计其次生根数,利用185对SSR标记对其进行基因型分析,采用TASSLE软件的GLM和MLM模型进行标记与性状的关联分析。结果表明,两种模型共同关联到32个显著标记位点,分布于14条染色体上。其中Barc81(1BL)、Wmc617(4DS)和Gwm190(5DS)在不同环境下表现稳定,且前人未曾报道。进一步对稳定位点进行有利等位变异分析,共挖掘出3个有利等位变异,其中Barc81-A180增效效应最大,同时鉴定出烟农24、烟农2415及冀麦34等20份材料携带有利等位变异。     

Tipping Points in Seaweed Genetic Engineering: Scaling Up Opportunities in the Next Decade

Seaweed genetic engineering is a transgenic expression system with unique features compared with those of heterotrophic prokaryotes and higher plants. This study discusses several newly sequenced seaweed nuclear genomes and the necessity that research on vector design should consider endogenous promoters, codon optimization, and gene copy number. Seaweed viruses and artificial transposons can be applied as transformation methods after acquiring a comprehensive understanding of the mechanism of viral infections in seaweeds and transposon patterns in seaweed genomes. After cultivating transgenic algal cells and tissues in a photobioreactor, a biosafety assessment of genetically modified (GM) seaweeds must be conducted before open-sea application. We propose a set of programs for the evaluation of gene flow from GM seaweeds to local/geographical environments. The effective implementation of such programs requires fundamentally systematic and interdisciplinary studies on algal physiology and genetics, marine hydrology, reproductive biology, and ecology.     

直播稻生产概况与品种选育策略

近年,直播稻面积在我国迅速扩大。本文结合国内外直播稻生产概况,指出了直播稻在抗倒伏、出苗率、耐冷性、防治杂草以及生育期等方面存在的问题,提出了培育“生育期适中、抗倒伏、耐低温、耐低氧萌发”的适合直播的水稻新品种选育策略。     

卷丹百合黑斑病病原鉴定及生物学特性研究

随着卷丹百合种植面积的扩大,卷丹百合叶部真菌性病害也越来越严重,尤其在2014年6~7月份,由于降水偏多,卷丹百合叶部病害大发生,6月中旬重病田卷丹百合枯死株率达50%~70%,部分田块卷丹百合地上部全部枯死。从卷丹百合发病叶片分离得到病原菌,进行致病性鉴定、孢子形态观察、18S rDNA序列分析,生物学特性研究,结果表明,该病原菌为半知菌链格孢（ Alternaria alternata）。该菌菌丝生长致死温度为55℃;适宜 pH为6~7;在供试的几种碳、氮源中,最适的碳源是麦芽糖,最适的氮源是酵母。     

植物组织培养:最新进展和潜在的应用(英文)

植物组织培养体系在基础研究和商业应用中具有巨大的潜能,例如园艺产业。组织培养过程伴随着一系列关于形态学、生理学、生物化学、分子和表观遗传的改变。分子水平的改变主要包括基因突变、DNA重组、染色体变异和表观遗传调控(DNA甲基化、组蛋白修饰、染色质重塑、小RNA调节)。这些改变被认为能促进外植体对培养环境的适应并有益于随后的形态发生。目前,组培已在商业应用和细胞生物学、遗传学、生物化学等基本研究中发挥了重要作用。本文重点介绍了植物组织培养的原理概念、培养基的制作、外植体的选择、各种激素的作用机理、植物离体快速繁殖的3大难题(外植体的污染、褐变、试管苗的玻璃化)以及防止措施,并详细阐述了植物离体快繁、无病毒苗木培育、培养细胞突变体、人工种子和离体培养期间分子水平的变化。     

耐铜菌株TLSB2-K的鉴定及其铜富集能力测定

[目的]研究菌株TLSB2-K的铜耐性以及其铜富集能力的特性.[方法]通过形态观察、革兰氏染色和16S rDNA序列比对,对前期分离的菌株TLSB2-K进行了鉴定,并采用振荡培养法,探讨了温度、pH值和渗透压对菌株生长的影响,以及铜胁迫下菌株对铜的耐性及富集能力.[结果]TLSB2-K属于蜡样芽孢杆菌(Bacillus cereus),最适生长条件为:温度为27℃、pH值为7、渗透压为1.1％ NaC1.铜浓度100～500 mg/L范围内,菌体生长良好,铜浓度在100～400 mg/L范围内,菌体铜含量随着铜浓度的升高而增加,当铜浓度400 mg/L胁迫培养30 h,菌体铜含量达到最大值2 250mg/kg;菌株的最高铜耐受浓度为700 mg/L.[结论]菌株TLSB2-K具有较强的铜耐性和较高的铜富集能力,具有重要的理论研究和工程应用价值.     

ISSR-Based Molecular Characterization of an Elite Germplasm Collection of Sweet Potato （Ipomoea batatas L.） in China

To determine the genetic diversity and population structure of sweet potato accessions cultivated in China, and to establish the genetic relationships among their germplasm types, a representative collection of 240 accessions was analyzed using inter-simple sequence repeat （ISSR） markers. The mean genetic similarity coefifcient, Nei’s gene diversity, and shared allele distance of tested sweet potato accessions were 0.7302, 0.3167 and 0.2698, respectively. The 240 accessions could be divided into six subgroups and ifve subpopulations based on neighbor-joining （NJ） clustering and STRUCTURE results, and obvious genetic relationships among the tested sweet potato accessions were identiifed. The marker-based NJ clustering and population structure showed no distinct assignment pattern corresponding to lfesh color or geographical ecotype of the tested sweet potato germplasm. Analysis of molecular variance （AMOVA） revealed small but signiifcant difference between white and orange-lfeshed sweet potato accessions. Small but signiifcant difference were also observed among sweet potato accessions from the Southern summer-autumn sweet potato region, the Yellow River Basin spring and summer sweet potato region and the Yangtze River Basin summer sweet potato region. This study demonstrates that genetic diversity in the tested sweet potato germplasm collection in China is lower than that in some reported sweet potato germplasm collections from other regions. Pedigree investigations suggest that more diverse Chinese sweet potato varieties should be formed by broadening the selection scope of breeding parents and incorporating the introduced varieties into future breeding programs.     

Molecular Mapping of a Stripe Rust Resistance Gene YrH9020a Transferred from Psathyrostachys huashanica Keng on Wheat Chromosome 6D

Stripe rust （yellow rust）, caused by Puccinia striiformis f. sp. tritici （Pst）, is one of the most devastating diseases of wheat throughout the world. H9020-1-6-8-3 is a translocation line originally developed from interspeciifc hybridization between wheat line 7182 and Psathyrostachys huashanica Keng and is resistant to most Pst races in China. To identify the resistance gene（s） in the translocation line, H9020-1-6-8-3 was crossed with susceptible cultivar Mingxian 169, and seedlings of the parents, F1, F2, F3, and BC1 generations were tested with prevalent Chinese Pst race CYR32 under controlled greenhouse conditions. The results indicated that there is a single dominant gene, temporarily designated as YrH9020a, conferring resistance to CYR32. The resistance gene was mapped by the F2 population from Mingxian 169/H9020-1-6-8-3. It was linked to six microsatellite markers, including Xbarc196, Xbarc202, Xbarc96, Xgpw4372, Xbarc21, and Xgdm141, lfanked by Xbarc96 and Xbarc202 with at 4.5 and 8.3 cM, respectively. Based on the chromosomal locations of these markers and the test of Chinese Spring （CS） nullitetrasomic and ditelosomic lines, the gene was assigned to chromosome 6D. According to the origin and the chromosomal location, YrH9020a might be a new resistance gene to stripe rust. The lfanking markers linked to YrH9020a could be useful for marker-assisted selection in breeding programs.