裸子植物DNA条形码ITS2高通用性引物的筛选

DNA条形码技术是利用标准DNA片段进行准确快速鉴定物种的一种方法,理想的DNA条形码片段应具有高通用性。虽然核糖体DNA内部转录间隔区II（ITS2）被建议作为种子植物有效的DNA条形码,但目前裸子植物还没有通用性高的引物可用。为获得高通用性的ITS2引物,本研究基于裸子植物55个属的5．8S基因的保守序列区设计了3个正向引物,与已有的ITS反向引物组合,组成了7对ITS2引物进行通用性的评价。选取了裸子植物8目、12科和40属的56个种用于本文的研究。引物组合5．8SR／ITS4、5．8SRa／ITS4和5．8SF2／S3R因为在科水平评价中通用性低或者产生的PCR产物有双带,因而排除在全部物种水平上进一步评价。其余4对引物（GYM-5．8SF1／ITS4、GYM-5．8SFl／S3R、GYM-5．8SF2／ITS4和S2F／S3R）在56个物种的PCR检测中,均有100％的扩增率。基于PCR产物的亮度、序列质量和正反向引物覆盖率的综合评价,建议引物GYM_5．8SF2／ITS4作为裸子植物条形码片段ITS2最好的通用引物。     

DNA条形码：物种分类和鉴定技术

当前,一项称为“生命的条形码”计划正在欧美等国展开,其目的是实现对地球上现存的约1000万物种进行快速和准确的鉴定。DNA条形码是一种利用短的DNA序列对物种进行鉴定的技术。对DNA条形码的概念和原理进行了介绍,举例说明了其在物种分类、遗传多样性及物种鉴定研究中广泛的利用价值,阐述了当前该领域的研究现状,对未来的发展方向进行了展望。     

地衣的ITS序列系统发育分析和DNA条形码的初探

目的:构建出地衣植物核糖体rDNA(nrDNA)的ITS序列的系统发育树并探讨地衣植物的DNA条形码.方法:以黑龙江五大连池风景区的地衣植物为材料,采用特异性引物对地衣植物的ITS序列进行Pcr扩增,直接对其Pcr产物进行测序,利用MEGA4.0软件建立地衣植物的ITS序列的系统发育树.结果:根据系统发育分析得出一致性指数CI和维持性指数RI分别为0 5356和0.6602,相同属地衣的样本间即种内的遗传距离 和不同属的样本间即种间的遗传距离(K-2-P)平均值分别为0.030和0.600,种间距离大于种内距离.结论:根据地衣植物样本间的遗传距离(K-2-P)的分析,得出核糖体rDNA的ITS基因对地衣近缘属的分类鉴定上具有一定的参考价值,建议作为地衣分类鉴定的条形码的测试片段.     

中国蜡盘衣属3新记录种

根据形态、解剖特征和化学特征,报道了蜡盘衣属（Biatora）中国新记录3种：阿拉斯加蜡盘衣（B.alaskana）、浅红蜡盘衣（B.alborufidula）和长孢蜡盘衣（B.longispora）,并编制了中国蜡盘衣属已知种的检索表。     

基于线粒体COⅠ基因DNA条形码的中国鲚属物种有效性分析

分析了150尾刀鲚Coilia nasus、湖鲚C.nasus taihuensis、短颌鲚C.brachygnathus、七丝鲚C.grayii及凤鲚C.mystus个体的COⅠ基因DNA条形码序列变异。结果显示,150条COⅠ基因条形码序列包含63种单倍型,单突变位点主要集中在100bp和600bp附近。刀鲚、短颌鲚和湖鲚群体间的遗传距离在0.253%～0.557%之间,显著低于COⅠ基因DNA条形码鉴别不同物种2%的遗传距离阈值,表明这3个群体应为同一物种。但是凤鲚两群体间的遗传距离为5.08%,大于2%的鉴别阈值,显示凤鲚两群体可能达到了种或亚种级差异水平。以日本鳀Engraulisjaponicus为外群,用邻接法、最大简约法和最大似然法构建了分子系统树显示,刀鲚、湖鲚和短颌鲚群体聚在一起,未能各自形成单系;凤鲚根据地理分布聚为两支;七丝鲚则聚成单系。研究表明COⅠ基因条形码技术可用于我国鲚属物种的鉴定。     

扫描生命条码 鉴定物种身份

自从林奈创立双命名法以来的250年中,170多万种生物已经被分类及命名。然而,这只是地球上估计现存的1000万～1亿种生物中的很小一部分,按照这个分类速度推测下去,还需要1500年～1．5万年的时间才能将所有的分类鉴定工作完成。     

2种块菌的物种分子鉴定与系统地位分析

以采自内蒙古贺兰山地区的2种块菌为实验材料,分别运用形态学和分子生物学方法进行物种鉴定,并通过与GenBank数据库信息比对,利用Mega5.1软件构建系统进化树,分析其进化关系并确定2种块菌的进化地位。结果表明:两菌株子囊果都为地下生;其中,菌株order-a为灰黄色,近球形到不规则形,较硬,表面被覆微绒毛;菌株tuber-b呈黄褐色,质地均匀,表面有疣状物,顶端呈凹陷状,全株带有干果般特殊的香气。经分子生物学方法分析认为菌株order-a为块菌属的一种,tuber-b为冬块菌(Tuber brumale),并初步确定为内蒙古新记录种。     

rDNA ITS序列在ACCC真菌鉴定中的应用

【目的】真菌无处不在,并与人类生活紧密相关。真菌的鉴定是科学研究和资源开发利用的基础。本研究从中国农业微生物菌种保藏管理中心(ACCC)随机选取已经定名的112株库藏真菌菌株作为实验材料,通过DNA测序,评估核糖体DNA内转录间隔区(rDNA ITS)序列在真菌属级鉴定上的应用。【方法】采用真菌DNA条形码rDNA ITS的序列测定和在GenBank中查寻比对的方法,对这些菌株进行属水平的鉴定复核。【结果】通过研究,供试菌株中有80株的属名与原鉴定相符,同时表明序列中套峰的情况降低与Gen Bank中序列比对的相似性。【结论】rDNA ITS序列测定法可以用于真菌菌株进行属水平的鉴定复核,国家菌种保藏机构应对已入库保藏和即将入库的所有真菌菌株都进行属水平的鉴定复核,并对菌株鉴定结果作审慎处理,原定名的名称及其变更历史应以"曾用名"在数据库中保留。     

基于ITS条形码序列的刺桐姬小蜂分子鉴定

【目的】刺桐姬小蜂Quadrastichus erythrinae Kim体型小,传统的形态学鉴定方法难以快速准确识别。【方法】本研究测定了刺桐姬小蜂的rDNA ITS1和ITS2序列,根据18S rDNA部分序列,利用MEGA的最大相似法(Maximum Likehood)构建系统发育树。根据刺桐姬小蜂ITS1和ITS2序列设计了特异引物,应用特异引物对单只刺桐姬小蜂进行PCR扩增,可稳定地扩增出明显的目的DNA条带。【结果】研究表明,基于ITS基因的DNA条形码技术可以用于刺桐姬小蜂的快速准确鉴定。【结论】因此,采用ITS1和ITS2区的特异性引物可对刺桐姬小蜂进行快速分子鉴定。     

基于ITS DNA条形码技术的牛至及其混伪品鉴定研究

目的:采用ITS DNA条形码技术鉴定牛至(Origanum vulgare L.)及其混伪品.方法:试剂盒法提取样品基因组DNA,通用引物5F-4R扩增ITS序列,Sanger测序法双向测序.使用BLAST法、遗传距离Kimura双参数模型法、单核苷酸多态性分析、邻近树4种不同方法对牛至及其混伪品74条ITS序列进行...     

A DNA barcoding approach for identification of hidden diversity in Parmeliaceae (Ascomycota): Parmelia sensu stricto as a case study

Accurate specimen identification is challenging in groups with subtle or scarce taxonomically diagnostic characters, and the use of DNA barcodes can provide an effective means for consistent identification. Here, we investigate the utility of DNA barcode identification of species in a cosmopolitan genus of lichen‐forming fungi, Parmelia (Parmeliaceae). Two hundred and two internal transcribed spacer (ITS) sequences generated from specimens collected from all continents, including Antarctica, were analysed, and DNA barcodes of 14 species of Parmelia s.s. are reported. Almost all species show a barcode gap. Overall, intraspecific divergence values were lower than the threshold previously established for Parmeliaceae. However, the mean and range were elevated by deep barcode divergences in three species, indicating the likely occurrence of overlooked species‐level lineages. Here, we provide a DNA barcode reference library with well‐identified specimens sampled worldwide and sequences from most of the type material to enable easy and fast accurate sample identification and to assist in uncovering overlooked species in Parmelia s.s. Further, our results confirm the efficiency of the ITS region in the identification of species of Parmelia s.s. © 2015 The Linnean Society of London, Botanical Journal of the Linnean Society, 2016, 180 , 21–29.     

Testing the potential of proposed DNA barcodes for species identification of Zingiberaceae

In 2009, the Consortium for the Barcode of Life (CBOL) recommended the combination of rbcL and matK as the plant barcode based on assessments of recoverability, sequencing quality, and levels of species discrimination. Subsequently, based on a study of more than 6600 samples belonging to 193 families from seven phyla, the internal transcribed spacer (ITS) 2 locus was proposed as a universal barcode sequence for all major plant taxa used in traditional herbal medicine. Neither of these two studies was based on a detailed analysis of a particular family. Here, Zingiberaceae plants, including many closely related species, were used to compare the genetic divergence and species identification efficiency of ITS2, rbcL, matK, psbK-psbI, trnH-psbA, and rpoB.The results indicate that ITS2 has the highest interspecific divergence and significant differences between inter- and intraspecific divergence, whereas matK and rbcL have much lower divergence values. Among 260 species belongingto 30 genera in Zingiberaceae, the discrimination ability of the ITS2 locus was 99.5% at the genus level and 73.1% at the species level. Thus, we propose that ITS2 is the preferred DNA barcode sequence for identifying Zingiberaceae plants.     

Developing DNA barcodes for species identification in Podophylloideae (Berberidaceae)

Species of Podophyllum, Dysosma, Sinopodophyllum, and Diphylleia, genera from Podophylloideae of Berberidaceae, have long been used in traditional herbal medicine in East Asia and/or North America. Accurate identification of the species of these four genera is crucial to their medicinal uses. In this study, we tested the utility of nine barcodes (matK, rbcL, atpH-atpI, rpl32-trnL^UAG, rps18-clpp, trnL-trnF, trnL-ndhJ, trnS-trnfM, and internal transcribed spacer (ITS)) to discriminate different species of Podophylloideae. Thirty-six individuals representing 12 species of Podophylloideae were collected from different locations in China, Japan, and North America. We assessed the feasibility of amplification and sequencing of all markers, examined the levels of the barcoding gap based on DNA sequence divergence between ranges of intra- and interspecific variation using pairwise distances, and further evaluated successful identifications using each barcode by similarity-based and tree-based methods. Results showed that nine barcodes, except rps18-clpp, have a high level of primer universality and sequencing success. As a single barcode, ITS has the most variable sites, greater intra- and interspecific divergences, and the highest species discrimination rate (83%), followed by matKwhich has moderate variation and also high species discrimination rates. However, these species can also be discriminated by ITS alone, except Dysosma versipellis (Hance) M. Cheng ex T. S. Ying and D. pleiantha (Hance) Woodson. The combination of ITS + matK did not improve species resolution over ITS alone. Thus, we propose that ITS may be used as a sole region for identification of most species in Podophylloideae. The failure of ITS to distinguish D. versipellis and D. pleiantha is likely attributed to incomplete lineage sorting due to recent divergence of the two species.     

Testing DNA barcodes in closely related species of Curcuma (Zingiberaceae) from Myanmar and China

The genus Curcuma L. is commonly used as spices, medicines, dyes and ornamentals. Owing to its economic significance and lack of clear‐cut morphological differences between species, this genus is an ideal case for developing DNA barcodes. In this study, four chloroplast DNA regions (matK, rbcL, trnH‐psbA and trnL‐F) and one nuclear region (ITS2) were generated for 44 Curcuma species and five species from closely related genera, represented by 96 samples. PCR amplification success rate, intra‐ and inter‐specific genetic distance variation and the correct identification percentage were taken into account to assess candidate barcode regions. PCR and sequence success rate were high in matK (89.7%), rbcL (100%), trnH‐psbA (100%), trnL‐F (95.7%) and ITS2 (82.6%) regions. The results further showed that four candidate chloroplast barcoding regions (matK, rbcL, trnH‐psbA and trnL‐F) yield no barcode gaps, indicating that the genus Curcuma represents a challenging group for DNA barcoding. The ITS2 region presented large interspecific variation and provided the highest correct identification rates (46.7%) based on BLASTClust method among the five regions. However, the ITS2 only provided 7.9% based on NJ tree method. An increase in discriminatory power needs the development of more variable markers.     

Prospects for discriminating Zingiberaceae species in India using DNA barcodes

We evaluated nine plastid(matK, rbcL, rpoC1, rpoB,rpl36-rps8, ndhJ, trnL-F, trnH-psbA, accD) and two nuclear(ITS and ITS2) barcode loci in family Zingiberaceae by analyzing 60 accessions of 20 species belonging to seven genera from India.Bidirectional sequences were recovered for every plastid locus by direct sequencing of polymerase chain reaction(PCR)amplicons in all the accessions tested. However, only 35(58%)and 40 accessions(66%) yielded ITS and ITS2 sequences,respectively, by direct sequencing. In different bioinformatics analyses, matK and rbcL consistently resolved 15 species(75%)into monophyletic groups and five species into two paraphyletic groups. The 173 ITS sequences, including 138 cloned sequences from 23 accessions, discriminated only 12 species(60%), and the remaining species were entered into three paraphyletic groups. Phylogenetic and genealogic analyses of plastid and ITS sequences imply the possible occurrence of natural hybridizations in the evolutionary past in giving rise to species paraphyly and intragenomic ITS heterogeneity in the species tested. The results support using matK and rbcL loci for barcoding Zingiberaceae members and highlight the poor utility of ITS and the highly regarded ITS2 in barcoding this family, and also caution against proposing ITS loci for barcoding taxa based on limited sampling.     

中国石鳞衣属（石鳞衣科）地衣一新种

通过形态学、解剖学、化学与分子系统学相结合的方法对采自巴音布鲁克自然保护区的地衣进行分类学研究,发现石鳞衣属地衣一新种——白缘石鳞衣Gypsoplaca albimarginata。新种的主要特征为地衣体具白色边缘、假根,子囊盘红褐色、镶嵌在鳞片表面。本研究对该种进行了详细的形态特征描述,并与其相似种进行了比较和讨论。     

Assessment of candidate plant DNA barcodes using the Rutaceae family

DNA barcoding is a rapidly developing frontier technology that is gaining worldwide attention.Here,seven regions (psbA-trnH,matK,ycf5,rpoC1,rbcL,ITS2,and ITS) with potential for use as DNA barcodes were tested for their ability to identify 300 samples of 192 species from 72 genera of the family Rutaceae.To evaluate each barcode’s utility for species authentication,PCR amplification efficiency,genetic divergence,and barcoding gaps were assessed.We found that the ITS2 region exhibited the highest inter-specific divergence,and that this was significantly higher than the intra-specific variation in the "DNA barcoding gap" assessment and Wilcoxon two-sample tests.The ITS2 locus had the highest identification efficiency among all tested regions.In a previous study,we found that ITS2 was able to discriminate a wide range of plant taxa,and here we confirmed that ITS2 was also able to discriminate a number of closely related species.Therefore,we propose that ITS2 is a promising candidate barcode for plant species identification.     

基于种特异性COI引物（SS-COI）的桉树枝瘿姬小蜂A、B隐种快速鉴定技术

隐种A和隐种B是桉树枝瘿姬小蜂Leptocybe invasa两种重要的全球入侵隐种,对多国林业生产造成了严重危害。由于桉树枝瘿姬小蜂体型微小,且无法从形态上区分隐种类型,给该害虫的防治造成困难。本研究基于线粒体DNA细胞色素C氧化酶亚基I（mtDNA COI）基因序列的种特异性（species-specific COI,SS-COI）PCR方法,研究桉树枝瘿姬小蜂隐种快速分子检测技术。基于隐种A、B的COI序列分别设计特异性SS-COI引物各1对（AF/AR和BF/BR）。使用这两对引物扩增同一桉树枝瘿姬小蜂样品DNA,即可有效进行隐种鉴定,同时两对引物也能互相验证鉴定结果。引物鉴定灵敏性检测结果显示,AF/AR与BF/BR均具有较高的鉴定灵敏性,其对DNA的有效鉴定浓度阈值分别为11.42 pg/μL和28.32 pg/μL。本研究开发的桉树枝瘿姬小蜂隐种A、B的快速鉴定方法解决了桉树枝瘿姬小蜂入侵地区隐种鉴别的难题,极大缩短鉴定时间、降低鉴定费用,为进一步探究桉树枝瘿姬小蜂隐种A、B的生物学差异以及它们对不同抗性品种桉树的适应能力提供技术参考。     

CO1在侧耳属物种快速鉴定中的应用

以侧耳属Pleurotus15个种的15个菌株为材料,根据GenBank上侧耳属细胞色素c氧化酶亚基Ⅰ基因（cytochrome c oxidase subunit 1 gene,CO1）序列信息,设计引物CO332F、CO332R,进行第一轮PCR扩增,结果显示所有菌株都能得到单一条带,根据条带大小,15个菌株可分为4组。随后针对每个种设计特异性引物,进行第二轮PCR扩增,结果显示每个菌株只有在自己特异的引物中出现目的条带。通过两轮扩增,根据扩增条带的大小和有无,即可对15个种进行快速鉴定。     

FTA-DNA直接提取法在病原真菌分子鉴定中的应用

目的建立并评价FTA-DNA直接提取法在病原真菌分子鉴定中的应用。方法采用whatman FTA-DNA直接提取法从25个不同种属的45株培养的菌株和6例临床标本中提取病原真菌DNA,用于病原真菌的测序鉴定。配制不同浓度的孢子悬液探索该方法的检测限和安全性。结果 45株菌株扩增后均能得到1条清晰的DNA扩增片段,并成功测序。应用该方法亦成功从腹水、胸水、口腔拭子、宫颈拭子来源的临床标本中直接提取DNA并成功鉴定病原真菌。该DNA提取方法联合降落PCR能检测到1.0×103个cell/mL的孢子悬液,1.0×104个cell/mL及以下浓度的孢子悬液可以被FTA卡完全灭活。结论 FTA-DNA直接提取法可快速有效地从培养的菌株及部分临床标本中提取并保存病原真菌DNA,用于病原真菌的测序鉴定。