白梨和砂梨S基因型确定及S34新基因的分离

梨是配子体型自交不亲和植物,确定不同品种的S基因型是科学杂交授粉及提高梨产量和品质的基础。本文根据砂梨S1-9等位基因一级结构特征,设计特异引物PF和PR,以白梨（Pyrus bretschneideri）种鹅梨（Pyrus bretschneideri‘Eli’）和砂梨（Pyrus pyrifolia）品种博多青（Pyrus pyrifolia‘Hakataao’）的叶片基因组DNA为模板,通过PCR·RFLP系统检测、克隆测序以及生物信息学分析,分离鉴定了它们的片段大小相似的2条S等位基因,从中获得1条新的S基因,命名为S34-RNase基因,并确定了这2个梨品种的S基因型,分别为鹅梨S13S34和博多青S22S34。     

中国梨2个自交不亲和新等位基因(S等位基因)的分子鉴定

自交不亲和是显花植物的一种重要生殖生理现象,为探明中国梨的自交不亲和特性,对‘锦香’(Pyrus bretschneideri cv. Jinxiang)和‘鹅酥’(Pyrus bretschneideri cv. Esu)2个中国梨品种进行了基因组PCR特异扩增、S基因序列分析及田间杂交授粉试验。结果确定它们各含1个新S-RNA酶基因,分别命名为S37-和S38-RNase,GenBank序列号为DQ839238和DQ839239。生物信息学分析结果表明,S37-和S38-RNA酶的推导氨基酸序列与S1-至S36-RNA酶36个梨S基因具有相同的、高度保守的C1和C2区,但其高变区与S1-至S36-RNA酶差异较大,其中与S15的差异最小,只有3个氨基酸不同。在推导的氨基酸水平上,S37与S38有96%的序列相似性,但两者与S15的相似性更高,皆为98%,与S32的相似性最低,都只有63%;S37和S38的内含子较大,分别为786bp和723bp,与S15的777bp大小接近。最后,经分析验证确定‘锦香’和‘鹅酥’的S基因型分别为S34S37和S15S38。     

中国梨品种S基因型鉴定的初步研究

采用PCR技术和聚丙烯酰胺凝胶电泳法对6个中国梨品种的s基因型进行了鉴定研究,并与已知S基因型的日本梨品种进行了比较。研究结果表明,供试的6个中国梨品种S基因型均不相同,‘西子绿’、‘金花’和‘金水酥’各包含了S1～S7以外的新的S基因,为这些品种田间授粉品种的选配提供了参考。     

基于cDNA芯片的梨品种S基因型鉴定及新S-RNase基因进化分析

梨品种S基因型鉴定对梨栽培中授粉品种选择和遗传育种都具有重要意义。本研究利用梨S-RNase基因荧光标记的特异引物PCR扩增获得梨品种荧光标记的cDNA特异产物;进一步完善梨S-RNase基因cDNA芯片,以被检测梨品种cDNA特异序列与梨S-RNase基因cDNA芯片杂交检测不同梨品种S基因型,并发现新的S-RNase基因。结果表明:利用梨S-RNase基因cDNA芯片鉴定了泸定王皮梨、兴山24号、弥渡百合等35个未知S基因型梨品种,确定了各品种的S基因型。结合PCRRFLP及DNA克隆和测序等技术,发现了7个新的S-RNase基因资源,获得了新S-RNase基因序列。序列分析表明各新S-RNase基因均具有S-RNase基因特异区域序列的典型特征;进化分析显示7个新S-RNase基因主要属于蔷薇科苹果亚科S-RNase类群,且存在种间和属间比种内和属内进化关系更近的现象。7个新的S基因分别命名为:PpS_(53)(Pyrus pyrifolia S53)、PpS_(54)、PpS_(55)、PpS_(56)、PpS_(57)、PpS_(58)和PpS_(59),GenBank登录号分别为:KX581753、KX581754、KX581755、KX581756、KX581757、KX581751和KX581752。     

基于苹果EST-SSR的梨种质资源遗传多样性分析

利用来自苹果的8对EST-SSR标记对48份梨(Pyrus)种质资源进行遗传多样性研究,以分析其在梨属植物上的通用性.结果表明,8对EST-SSR引物在供试材料上均能扩增出与苹果大小相似的产物,所有引物共检测到140个基因位点,其中多态性位点129个,多态性比例为92.14%,并且可成功区分不同品种.根据EST-SSR标记所揭示的多态性和UP-GMA法聚类分析,48份梨种质资源在相似系数0.62处可分为东方梨和西方梨两个种群,而中国的白梨(Pyrus bretschneideri Rehd.)、砂梨(P.pyrifolia Burm.f.Nakai)和秋子梨(P.ussuriensis Maxim.)相互交错在一起,没有独自成组.可见,苹果的EST-SSR标记在梨上具有高度的可转移性,可应用于梨属植物的资源评价及遗传关系研究.     

梨自交不亲和基因cDNA芯片杂交条件优化及应用北大核心

[目的]优化梨自交不亲和基因(S-RNase或S基因)c DNA芯片杂交条件,利用芯片检测梨品种S基因型。[方法]提取梨品种雌蕊RNA,Cy3标记引物RT-PCR获得S基因荧光标记特异c DNA序列。设置不同杂交条件,用已知S基因型品种荧光标记的PCR产物在不同条件下分别与芯片杂交,杂交信号分析芯片杂交效果。用芯片优化杂交体系鉴定梨品种未知S基因型,DNA测序验证芯片鉴定结果。[结果]芯片杂交最佳条件:杂交温度42℃,杂交时间8~9 h,PCR纯化产物终浓度为200 ng·μl-1。优化杂交条件下芯片鉴定晚咸丰、秀水、丽江马占梨1、湘菊、木通梨、甘甜、弥渡小红梨、丽江大中古、金晶和弥渡火把等梨品种S基因型分别为:Pp S15Pp S52、Pp S4Pp S5、Pb S22Pp S37、Pp S1Pp S2、Pp S1Pp S3、Pp S13Pp S15、Pp S12Pb S42、Pb S21Pb S22、Pp S3Pp S60和Pp S5Pp S5。DNA测序验证各品种所含S基因与芯片鉴定结果一致。[结论]梨自交不亲和基因c DNA芯片优化杂交条件后可准确鉴定梨品种所含已鉴定的S基因资源。     

高温胁迫对‘黄冠’、‘翠玉’梨耐热生理指标及相关基因表达的影响

为探讨高温胁迫对梨树的影响,对2年生‘黄冠’(Pyrus pyrifolia‘Cuiguan’)、‘翠玉’(P.bretschneideri×P.pyrifolia)盆栽苗胁迫后叶片的抗氧化物质、抗氧化酶、渗透物质和激素的变化进行了测定,利用q RT-PCR分析了叶片中抗性基因的表达。结果表明,在高温胁迫下,梨树叶片的叶绿素含量明显下降,而MDA含量则持续上升;梨叶片中的POD和CAT活性总体呈下降趋势,但‘黄冠’的POD和CAT活性均高于‘翠玉’;PRO含量随胁迫时间延长逐渐增加;ASA含量表现出先上升后下降,且‘黄冠’的ASA含量高于‘翠玉’;IAA和ABA含量都随胁迫时间的延长呈下降趋势,但‘黄冠’的IAA和ABA含量比‘翠玉’高。q RT-PCR结果表明,叶片中相关基因的表达量与对应的ASA、IAA和ABA含量变化趋势基本一致。因此,‘黄冠’比‘翠玉’抗高温性能强,且高温处理第4天为‘黄冠’和‘翠玉’梨的生理变化转折点。     

24份甜樱桃材料自交不亲和S基因型鉴定

甜樱桃品种绝大部分自交不亲和,限制了甜樱桃的正确评价和合理利用,因此自交不亲和基因型的鉴定对于生产具有重要意义。以24个甜樱桃主栽品种为材料,用5对蔷薇科李属引物组合对24个甜樱桃品种进行了S等位基因的PCR扩增,克隆S基因的扩增片段,用核酸序列在Gen Bank上搜索,确定了5种S基因的核酸序列和大小。结果表明:Pru C2+Pru C4R引物组合扩增效果最好;在琼脂糖凝胶上位置相同的扩增带其核酸序列相同,是同一种S基因;5种S基因扩增片段的大小分别是S1为800 bp,S3为762 bp,S4为962bp,S5为300 bp,S6为456 bp,S9为650 bp;24个甜樱桃S基因型是红手球、早红宝石为S1S3,拉宾斯S1S4',红宝石S1S6,布鲁克斯S1S9,那翁S3S4,秦林、泰安大紫、先锋、早大果、丽珠、美早、5-106、左滕锦、桑提娜为S3S6,黑珍珠、红灯、萨米脱、秦樱为S3S9,胜利为S5S9,明珠、红蜜、雷尼、滨库为S6S9。     

‘黄花’梨及其芽变‘绿黄花’梨HHT基因克隆与表达分析

该试验以砂梨品种‘黄花’梨（果皮褐色）及其芽变‘绿黄花’梨（果皮绿色）盛花后第8周的果皮为试材,利用常规PCR和巢式PCR技术克隆了ω 羟基棕榈酸O 阿魏酰转移酶（ω hydroxypalmitate O feruloyl transferase, HHT）基因cDNA的全长,命名为 PpyHHT（登录号为KX131155）。序列分析结果表明,该基因开放阅读框（ORF）为1 335 bp,编码444个氨基酸。生物信息学分析显示,推定的PpyHHT蛋白质相对分子质量为49.91 kD,等电点是4.75,与白梨相似性高达98%,亲缘关系最近。实时荧光定量PCR（qRT PCR）表达分析显示,2种梨果皮中 PpyHHT基因在盛花后6~9周的4个转色关键期表达量不断变化,在‘黄花’梨果皮中的表达量明显高于‘绿黄花’梨。推测 PpyHHT基因可能参与砂梨果实褐色/绿色性状的形成。     

11个苹果新品种自交不亲和基因的分离与鉴定

以11个苹果品种为试验材料,根据保守氨基酸序列"FTQQYQ"和"anti-1/WⅠPNV"设计苹果自交不亲和基因引物,利用酶切分析和目的片段DNA测序方法鉴定了9个新的S-等位基因,将该9个S-等位基因分别标记为:S34-、S35-、S36-、S37-、S38-、S39-、S40-、S41-、S42-等位基因,在GeneBank中的接收号依次为:EU310474、EU391605、EU391606、EU391607、EU391609、EU391610、EU391611、EU391612、EU391613。11个苹果品种的自交不亲和基因型分别为:桑萨(S40S40)、芳明(S1S9),烟嘎1(S38S27)、红金嘎拉(S39S27)、烟嘎2(S38S27)、青9号(S41S42)、阿斯(S36S36)、皇家嘎拉(S37S27)、静香(S1S9S34)、高岭(S38S9)、红奥(S35S35)。     

梨种质资源对黑星病抗性评价

采用人工接种黑星病菌的方法,对国家果树种质兴城梨资源圃保存的197份梨种质资源进行了抗病性鉴定,结果表明:不同梨种类发病率差异很大,其中白梨和砂梨最易感病,秋子梨和种间杂交选育品种较易感病,新疆梨较抗病,西洋梨最抗病;对病情指数在各梨种类分布进行了分析;在白梨、砂梨、秋子等各系统分别筛选出黄鸡腿、甩梨、酸梨、锦香等一批抗病资源;对田间自然感病与人工接种感病结果进行了比较。     

Rapid identification of 1-aminocyclopropane-1-carboxylate (ACC) synthase genotypes in cultivars of Japanese pear (Pyrus pyrifolia Nakai) using CAPS markers

In Japanese pear (Pyrus pyrifolia Nakai), fruit storage potential is closely related to the amount of ethylene produced. We have developed a rapid and accurate method for analyzing genes involved in high ethylene production during fruit ripening in Japanese pear. This involves cleaved-amplified polymorphic sequences (CAPS) of two 1-aminocyclopropane-1-carboxylate (ACC) synthase genes (PPACS1 and PPACS2). Two CAPS markers (A for PPACS1 and B for PPACS2), associated with the amount of ethylene produced, were identified. Marker A was associated with high ethylene producers and marker B with moderate ethylene producers. The absence of these two markers enabled the identification of low ethylene producers. Using these markers, we have identified ethylene genotypes for 40 Japanese pear cultivars and two Chinese pear (P. bretschneideri) cultivars that are commercially important and used in breeding programs. Furthermore, we performed linkage analysis of these two genes in the F(2) population, which revealed that the recombination frequency between the two markers was 20.8 +/- 3.6%. This information is critical to the selection of parents and in breeding strategies to improve storage ability of Japanese pears.     

基于苹果基因组开发梨的多态性SSR引物

从NCBI网站获取‘金冠’苹果基因组数据,在每条染色体上随机设计4对共68对引物。利用梨品种‘黄冠’和‘莱阳茌梨’及其F1代杂交群体(共94个单株)对这些引物的应用性进行验证,同时分析了该群体遗传多样性。(1)引物扩增结果显示,有40对引物可以扩增出预期目的条带,占设计引物数量的58.82%,其中16对引物能够扩增出多态性条带。(2)群体遗传多样性分析结果显示,有16对多态性引物扩增产物的等位基因数平均为2.312 5,有效等位基因数平均为2.001 4,平均杂合度观测值、期望杂合度和香农指数分别为0.548 3、0.490 5和0.746 2,表明可以在梨上运用。研究证明,SSR位点在苹果与梨之间可以转移应用。     

Evolutionary analysis of S-RNase genes from Rosaceae species

Eight new cDNA sequences for S-RNases were cloned and analysed from almond (Prunus dulcis) cultivars of European origin, and compared to published sequences from other Rosaceae species. Insertions/deletions of 10-20 amino acid residues were detected in the RC4 and C5 domains of S-RNases from almond and sweet cherry. The S-RNases of the Prunus species and those of the genera Malus and Pyrus formed two distinct groups on phylogenetic analysis. Nucleotide substitutions were analysed in the S-RNase genes of these species. The S-genes of almond and sweet cherry have a lower Ka/Ks value than those of apple, pear and wild apple do. The fact that there is no fixed difference between the S-RNase genes of almond and sweet cherry, or between apple and pear, suggests that nucleotide substitutions only introduce transient polymorphism into the two groups, and rarely became fixed and contribute to divergence. Through the comparative study of 17 S-RNase genes from the genus Prunus and 18 from the genera Malus and Pyrus, some fixed nucleotide differences between the two groups were identified. These differences do not appear to be the result of selection for adaptive mutations, since the number of replacement substitutions is not significantly greater than the number of synonymous substitutions. S-RNase genes of almond and sweet cherry, and of apple and pear, showed little heterogeneity in nucleotide substitution rates. However, heterogeneity was observed between the two groups of S-alleles, with the Prunus alleles exhibiting a lower rate of non-synonymous substitutions than alleles from Malus and Pyrus. The evolutionary relationships between these species are discussed.     

不同基因型梨木质素代谢对石细胞含量和果实口感的影响

以五种基因型梨果实为材料,对石细胞团的大小、分布进行解剖学观察,并测定石细胞、木质素含量和木质素相关合成酶PAL、POD、PPO活性,探讨不同基因型梨果实木质素代谢对石细胞含量及口感的影响.结果表明,不同基因型梨木质素含量高时,石细胞含量也高,石细胞团相对较大,分布较密集,口感差.各基因型的梨木质素、石细胞含量和大小为...     

New findings in apple S-genotype analysis resolve previous confusion and request the re-numbering of some S-alleles

Apple trees display gametophytic self-incompatibility which is controlled by a series of polymorphic S-alleles. To resolve the discrepancies in S-allele assignment that appeared in the literature, we have re-examined the identity of S-alleles known from domestic apple cultivars. Upon an alignment of S-allele nucleotide sequences, we designed allele-specific primer pairs to selectively amplify a single S-allele per reaction. Alternatively, highly similar S-alleles that were co-amplified with the same primer pair were discriminated through their distinct restriction digestion pattern. This is an extension of our previously developed allele-specific PCR amplification approach to reveal the S-genotypes in apple cultivars. Amplification parameters were optimised for the unique detection of the 15 apple S-alleles of which the nucleotide sequences are known. Both the old cultivars with a known S-genotype and a number of more common cultivars were assayed with this method. In most cases, our data coincided with those obtained through phenotypic and S-RNase analysis. However, three S-alleles were shown to relate to RNases that were previously proposed as being encoded by distinct S-alleles. For another S-allele the corresponding gene product has not been discriminated. Consequently, we propose the re-numbering of these four S-alleles. Furthermore, two alleles that were previously identified as S(27a) and S(27b) now received a distinct number, despite their identical S-specificity. To ease widespread future analysis of S-genotypes, we identified common cultivars that may function as a witness for bearing a particular S-allele. We discuss the assignment of new S-alleles which should help to avoid further confusion.     

Genomic characterization of self-incompatibility ribonucleases in the Central Asian pear germplasm and introgression of new alleles from other species of the genus Pyrus

The Pyrus species exhibit the so-called S-RNase-based gametophytic self-incompatibility system, which is considered to be the most widespread self-incompatibility system among flowering plants. In this study, 57 Iranian pear (Pyrus communis L.) domestic cultivars and wild genotypes, plus 21 European pear cultivars used as references, were genotyped adopting a PCR-based genotyping assay using consensus and allele-specific primers. The results revealed traces of significant genetic contribution in the Iranian traditional varieties and genotypes from other Pyrus species; the genetic contribution of Japanese pear clearly emerged with the detection of some Pyrus pyrifolia S-RNase alleles. Moreover, our results highlighted the presence of three new S-RNase alleles (named S₁₂₆, S₁₂₇, and S₁₂₈) that were not previously identified in P. communis, possibly introduced in the germplasm of cultivated pear through gene transfer from other cultivated or wild species.