Molecular Phylogeny of the “True Citrus Fruit Trees” Group (Aurantioideae, Rutaceae) as Inferred from Chloroplast DNA Sequence

The genus Citrus L. has a long controversial taxonomy history, and a well-resolved molecular phylogeny of the "True Citrus Fruit Trees"group in the future will provide new information for advancing breeding techniques and developing better conservation strategies. In the present study, three cpDNA fragments (TrnL-TrnF, PsbH-PetB, and TrnS-TrnG) of 30 genotypes chosen from the six genera of the "True Citrus Fruit Trees"group were analyzed. A molecular phylogenetic tree of the "True Citrus Fruit Trees"group was reconstructed based on plastid DNA sequences. The results confirmed that the "True Citrus Fruit Trees"group was monophyletic, and thereby the group was divided into genera as previously suggested based on morphological characters. The cpDNA data also suggested that Poncirus might be the first genus separated from the other five genera in the group. The genus Fortunella were of hybrid origin and Citrus might be as its putative paternal parent. The genera Microcitrus, Eremocitrus, and Clymenia were possibly monophyletic and their common ancestor might branch out from Citrus. Furthermore, the phylogenetic relationships within the Citrus genus were discussed.

木材分子考古研究进展

木材考古学研究是推动木质文物自然和历史信息挖掘、保护和修复的重要基础。近年来,随着古DNA捕获和测序技术的快速发展,从木质遗存中可获取古DNA信息,在木材解剖学基础上,创新开展以古DNA为核心的木材分子考古研究已成为木材考古学的前沿热点。本文首先对木材分子考古研究进行概述,从古DNA的保存和降解、获取以及数据处理和序列分析3方面归纳木材古DNA的研究进展,并指出古DNA因高度降解、含量极低和化学损伤特征导致其难于提取和信息解译的难题。然后总结木材分子考古在解读先民认知与利用森林资源方式、复原历史时期地域性森林植被类型和物种多样性以及重建古代树木应对气候和生境变化的微进化反应等方面的主要应用。最后提出该研究领域未来应优先开展的工作:1)建立考古木材标本库及其DNA信息数据库;2)研究不同时空维度下木材古DNA损伤及变化规律;3)构建稳定高效的木材古DNA提取及序列信息解译技术体系。通过进一步加强木材分子考古等多学科交叉研究,推动新理论、新方法、新技术在木材学和考古学领域的应用,为木质文物的用材树种识别、保护利用以及重建历史时期森林植被、环境气候与人类活动的耦合关系提供重要科学依据。

给定悬挂点个数的分子树的ISDD指数的极值

设G=(V (G),E (G))为n阶连通图,其顶点集为V (G),边集为E (G),用deg (x)表示顶点x的度,则图G的反对称分割指数为ISDD(G)=∑_(xy∈E(G))(deg(x)·deg(y)/deg(x)^(2)+deg(y)^(2))。本文主要采用不等式和分类讨论法对具有固定悬挂点的分子树的ISDD指数进行了研究,分别讨论了悬挂点个数为偶数和悬挂点个数大于等于3时分子树的ISDD指数的极值,分子树是指顶点度不超过4的树。首先,确定了当悬挂点个数为偶数时,分子树中反对称分割指数为最小值,此时,ISDD(MT)=1/2n-31/85p-1/10;其次,确定了当悬挂点个数大于等于3时,分子树中反对称分割指数为最大值,此时,ISDD(MT)=1/2n-9/65p-1/2,并刻画了达到ISDD指数极值的分子树。

关于我国林木育种向智能分子设计育种发展的思考

“作物育种4.0”的提出,为我国林木遗传育种指明了向智能分子设计育种发展的前进方向。本文提出了理想品种的概念及其智能设计实现条件,简要综述了我国林木遗传育种研究历史以及存在的问题,并提出了推动我国林木智能分子设计育种的发展对策等。林木遗传育种应该瞄准国家林业重大需求,有组织地选择重要树种系统布局,在推动树种高世代遗传改良及其利用的同时,准备系谱关系清晰的育种资源群体,做到等位变异有迹可循;解析重要性状遗传变异规律及其调控网络,实现基因调控有据可查;建立高效的多组学大数据整合分析以及育种群体构建、亲本选配和后代选择等分子设计育种技术方法体系,保证智能育种有“法”可依等。逐步解决我国林木遗传育种中存在的问题,为实施林木智能设计育种创造理想条件。在每一育种世代品种向理想品种选育的推进过程中,尽可能将智能分子设计育种的最新理论和技术成果应用于育种实践,选育出高产、优质、高抗的当前世代理想品种,满足国家林业发展的现实需要。

On Augmented Zagreb Index of Molecular Graphs

The augmented Zagreb index displays a good correlation with the formation heat of octanes and heptanes. The augmented Zagreb index of catacondensed hexagonal systems and molecular trees was discussed. By using the methods of analysis of graph structure and mathematical induction,the catacondensed hexagonal systems with extreme augmented Zagreb index were characterized.The lower bound for augmented Zagreb index of molecular trees with fixed numbers of pendent vertices was given,and the extremal trees were characterized. From these results,we can compare the formation heat of catacondensed hexagonal systems and molecular trees.

果树分子标记辅助育种研究进展

随着分子生物学的不断发展,分子标记在果树育种中发挥的作用也愈发重要。本文主要对不同果树育种的分子标记类型及分子标记在果树种质资源鉴定、抗性育种、无核育种、早熟育种、品质改良育种、分子遗传图谱构建与数量性状座位(QTL)基因定位等方面的应用进行了综述,为果树分子标记辅助育种提供参考。

叠氮丙啶-实时荧光聚合酶链式反应-高通量测序技术鉴定冷链食品中多种病原菌

目的 应用叠氮丙啶-实时荧光聚合酶链式反应-高通量测序技术鉴定冷链食品中多种病原菌,构建病原菌分子进化树。方法 以冷链食品中的沙门氏菌、金黄色葡萄球菌、蜡样芽胞杆菌、副溶血性弧菌、单核细胞增生李斯特氏菌5种病原菌作为研究对象,应用叠氮丙啶-实时荧光聚合酶链式反应技术作为冷链食品中病原菌检测初筛手段,应用微生物培养法以及生化鉴定仪器法进行方法比对与结果验证,运用高通量测序以及分子进化树构建作为冷链食品中所分离病原菌的种属地位确证方法。结果 叠氮丙啶-实时荧光聚合酶链式反应技术成功扩增了冷链食品中生活状态病原菌的特征性核酸片段,排除了死亡细菌以及阴性对照菌的干扰,病原菌检出限可达到1×10^(3)CFU/mL,一次反应可检测42份试样,可以在18 h内完成检测工作。在冷链食品中病原菌抽样检测调查中,随机采集的751份冷链食品,共检出62株病原菌,病原菌总体检出率为8.3%(62/751)。通过后续的16S rRNA测序以及葡萄球菌属、弧菌属以及李斯特菌属分子进化树的构建,成功溯源了金黄色葡萄球菌的污染来源并完成病原菌种属定位。结论 本方法特异性好、灵敏度高、检测通量高,为冷链食品及相关食品中病原菌的精确检测与溯源分析提供新的思路与方法。

红叶石楠叶斑病致病菌的分离与鉴定

【目的】为明确红叶石楠患叶斑病叶片的致病菌,以期为红叶石楠叶斑病的防控提供借鉴参考。【方法】2022年9月以福建省南平市武夷山市武夷学院采集的患病叶片为材料,利用传统微生物培养法分离纯化致病菌,进行柯赫氏法则验证,通过形态学鉴定和ITS序列分析明确致病菌的种类。【结果】从病叶中分离得到的菌株a在PDA培养基上呈白色絮状,有明显的轮纹,分生孢子为纺锤形,菌株a的ITS序列与NCBI数据库中小孢拟盘多毛孢属(Pestalotiopsis microspora,登录号:AY924271.1)的相似性为99%。菌株b在PDA培养基上呈白色蓬松状,有大量气生菌丝,孢子呈黑色球状,菌株b的ITS序列与NCBI数据库中稻黑孢属(Nigrospora oryzae,登录号:KT192348.1)的相似性为99%。接种菌株a和菌株b均能使离体叶片发病,且症状与供试叶片的症状相似。【结论】引发武夷学院红叶石楠叶斑病的病原物为小孢拟盘多毛孢菌和稻黑孢菌。

Characterization of Avian Influenza A(H7N9) Virus Prevalence in Humans and Poultry in Huai′an,China：Molecular Epidemiology,Phylogenetic,and Dynamics Analyses

Objective To trace the source of human H7N9 cases in Huai'an and elucidate the genetic characterization of Huai'an strains associated with both humans and birds in live poultry market.Methods An enhanced surveillance was implemented when the first human H7N9 case was confirmed in Huai'an.Clinical specimens,cloacal swabs,and fecal samples were collected and screened by real-time reverse transcription-polymerase chain reaction(RT-PCR) for H7N9 virus.The positive samples were subjected to further RT-PCR and genome sequencing.The phylodynamic patterns of H7N9 virus within and separated from Huai'an and evolutionary dynamics of the virus were analyzed.Results Six patients with H7N9 infection were previously exposed to live poultry market and presented symptoms such as fever(>38.0 °C) and headaches.Results of this study support the hypothesis that live poultry markets were the source of human H7N9 exposure.Phylogenetic analysis revealed that all novel H7N9 viruses,including Huai'an strains,could be classified into two distinct clades,A and B.Additionally,the diversified H7N9 virus circulated in live poultry markets in Huai'an.Interestingly,the common ancestors of the Huai'an H7N9 virus existed in January 2012.The mean nucleotide substitution rates for each gene segment of the H7N9 virus were(3.09-7.26)×10-3 substitutions/site per year(95% HPD:1.72×10-3 to 1.16×10-2).Conclusion Overall,the source of exposure of human H7N9 cases in Huai'an was live poultry market,and our study highlights the presence of divergent genetic lineage of H7N9 virus in both humans and poultry specimens in Huai'an.

The Exploration of Trimeresurus Divided to Multiple Genera Based on Molecular Systematics

According to the contradictions about classification on Trimeresurus between " China's Fauna" and international database,the rationality about Trimeresurus divided to multiple genera based on molecular systematics was discussed. The genetic distance was calculated by sequencing 12S gene of the original Trimeresurus snakes,including 80 individuals of 33 species; and the molecular phylogenetic tree was established by taking Hypnale hypnale as the outgroup. The results showed that the topological structures of ME tree and ML tree were basically consistent,and all of the species in the molecular trees were divided into 8 branches;and the difference of T. albolabris between Hainan and other locations is not obvious. The viewpoint that original Trimeresurus genera subdivided into 8 genera was more rational,and new authoritative reference books are expected to be published in China.

家猫感染东方次睾吸虫形态学特征及分子鉴定

目的了解家猫感染东方次睾吸虫的形态学及基因特征,为当地开展东方次睾吸虫病防控工作提供理论依据。方法采集浦城县感染有东方次睾吸虫囊蚴的麦穗鱼,剪碎囊蚴寄生处的鱼尾部肌肉,喂食2个月龄家猫。45 d后连续多天检测家猫粪便中的虫卵,直至发现虫卵后进一步深入检查。观察肝脏及胆囊变化和虫体寄生部位,捡出虫体置于生理盐水中,对虫体的形态学特征进行观察与鉴定描述。提取虫体基因组DNA,PCR扩增ITS基因序列,测序后在GenBank上进行BLAST比对,采用邻接法构建系统进化树。结果从胆囊和肝脏分离获得13条东方次睾吸虫。东方次睾吸虫为雌雄同体,虫体大小约为(1.95~2.86)mm×(0.61~0.93)mm;虫卵呈长椭圆形,似葵花籽状,虫卵大小约(28~32)μm×(16~18)μm。PCR结果显示,ITS基因序列扩增产物260 bp。BLAST比对结果显示,与国内已报道家鸭及黑天鹅感染的东方次睾吸虫(GenBank登入号分别为MT231323.1、MK482055.1、MK482052.1)的序列一致性均为99.62%。基于ITS基因的系统进化树显示,本研究分离获得的吸虫ITS序列属于次睾属,与东方次睾吸虫(GenBank登入号分别为HM347224、KX832894、MK482055、MT231323、KX857496、MK482052)属于同一个分支。结论从家猫分离的虫体经形态学及基因分析与文献报道的一致,鉴定为东方次睾吸虫。

Learning Probabilistic Models of Hydrogen Bond Stability from Molecular Dynamics Simulation Trajectories

Hydrogen bonds (H-bonds) play a key role in both the formation and stabilization of protein structures. H-bonds involving atoms from residues that are close to each other in the main-chain sequence stabilize secondary structure elements. H-bonds between atoms from distant residues stabilize a protein’s tertiary structure. However, H-bonds greatly vary in stability. They form and break while a protein deforms. For instance, the transition of a protein from a non-functional to a functional state may require some H-bonds to break and others to form. The intrinsic strength of an individual H-bond has been studied from an energetic viewpoint, but energy alone may not be a very good predictor. Other local interactions may reinforce (or weaken) an H-bond. This paper describes inductive learning methods to train a protein-independent probabilistic model of H-bond stability from molecular dynamics (MD) simulation trajectories. The training data describes H-bond occurrences at successive times along these trajectories by the values of attributes called predictors. A trained model is constructed in the form of a regression tree in which each non-leaf node is a Boolean test (split) on a predictor. Each occurrence of an H-bond maps to a path in this tree from the root to a leaf node. Its predicted stability is associated with the leaf node. Experimental results demonstrate that such models can predict H-bond stability quite well. In particular, their performance is roughly 20% better than that of models based on H-bond energy alone. In addition, they can accurately identify a large fraction of the least stable H-bonds in a given conformation. The paper discusses several extensions that may yield further improvements.

海南橡胶树炭疽病调查及喀斯特炭疽病菌的鉴定

天然橡胶是四大工业原料中唯一的可再生资源,由炭疽病菌侵染引起的橡胶树炭疽病是当前我国橡胶生产上最为严重的两大叶部病害之一。本研究通过调查海南省主栽橡胶树品种(系)及监测炭疽病发生流行情况,调查发现PR107和RRIM600种植面积最大,分别占51.06%(102000 hm^(2))和43.39%(86700 hm^(2));在对橡胶树炭疽病的随机踏查和固定监测中发现,该病在实生苗、嫁接苗、增殖苗、各主栽品种幼龄树和成龄胶园中全年均可发生,3—4月为盛发期;海南省橡胶树种植面积大,且品种(系)单一,因此炭疽病在适宜发病条件下易暴发流行。通过形态观察、致病性测定和多基因系统发育分析发现,分离自琼中县阳江农场苗圃橡胶树叶片上的菌株HCkHNQZ1736为喀斯特炭疽菌(Colletotrichum karstii),这是首次在海南省橡胶树上发现该类病菌。致病力评价发现其对PR107、RRIM600、热研7-33-97和大丰95四个主推品种均有强致病力。杀菌剂敏感性测定结果表明,菌株HCkHNQZ1736和分离自云南保山的同种菌株MeCkYN1705对咪鲜胺锰盐差异不显著且不具抗药性,EC_(50)分别为0.0784μg/mL和0.0775μg/mL。HCkHNQZ1736对多菌灵表现出高抗药性,EC_(50)达1107.2654μg/mL,而MeCkYN1705的EC_(50)仅为0.0554μg/mL。

基于rDNA序列分析的3种丛枝菌根真菌分子鉴定方法比较

【目的】比较基于rDNA序列分析的3种丛枝菌根(AM)真菌分子鉴定方法,为提高AM真菌在种水平分子鉴定的准确性提供参考。【方法】对从柑橘和甘蔗等广西地区主要作物的根际土壤中分离出的AM真菌菌株(编号为A6、B3和GY3-1)进行形态学鉴定,再通过巢式PCR分别扩增AM真菌的18S rDNA、28S rDNA及含ITS1、5.8S rDNA和ITS2的序列(简写为ITS1+5.8S+ITS2),分别将其测序结果与GenBank数据库进行比对,并构建系统发育进化树,再结合形态学鉴定结果比较基于3个rDNA序列分析分子鉴定方法的准确性。【结果】菌株A6、B3和GY3-1的形态特征分别与幼套近明球囊霉(Claroideoglomus etunicatum)、黏质隔球囊霉(Septoglomus viscosum)和摩西斗管囊霉(Funnelifor-mis mosseae)一致。基于18S rDNA序列,将菌株A6鉴定为近明球囊霉属(Claroideoglomus),菌株GY3-1鉴定为摩西斗管囊霉(F.moessae),菌株B3鉴定为黏质隔球囊霉(S.viscosum)。基于28S rDNA序列,将菌株A6鉴定为幼套近明球囊霉(C.etunicatum),菌株B3鉴定为黏质隔球囊霉(S.viscosum),菌株GY3-1鉴定为摩西斗管囊霉(F.moessae)。基于ITS1+5.8S+ITS2序列,将菌株A6鉴定为幼套近明球囊霉(C.etunicatum),菌株B3鉴定为黏质隔球囊霉(S.visco-sum),菌株GY3-1鉴定为摩西斗管囊霉(F.moessae)。而综合3种分子鉴定结果,菌株A6、B3和GY3-1分别鉴定为幼套近明球囊霉(C.etunicatum)、黏质隔球囊霉(S.viscosum)和摩西斗管囊霉(F.mosseae)。【结论】3种方式均可用于AM真菌的在种水平上的分子鉴定,以18S rDNA与28S rDNA为主的鉴定方法相对简单且快速,更适用于对AM真菌在属水平的鉴定;以ITS1+5.8S+ITS2为主的鉴定方法步骤较繁琐,但鉴定至种水平的准确性较高。3种方法的分析结果在一定程度上可互相补充,加强对AM真菌分子鉴定结果的准确性。

Molecular Cloning of a Chitinase Gene from the Ovotestis of Kuroda’s Sea Hare Aplysia kurodai

In this study, we report that we successfully cloned and sequenced a chitinase gene from the ovotestis of Kuroda’s sea hare Aplysia kurodai. By using reverse transcription-polymerase chain reaction (RT-PCR) and a system for the 5’ and 3’ rapid amplification of cDNA ends, we obtained a 1352 bp chitinase gene (AkChi) from the ovotestis of A. kurodai. AkChi contains a 1263 bp open reading frame that encodes 421 amino acids. The domain structure predicted from the deduced amino acid sequence was an N-terminal signal peptide and a catalytic domain of glycoside hydrolase (GH) family 18 chitinase. A comparative analysis of the deduced amino acid sequences of AkChi with those of the acidic mammalian chitinase of the California sea hare Aplysia californica revealed the highest homology at 83%. The purified chitinase from the ovotestis was digested by trypsin, and 119 residues of digested peptides were consistent with the deduced amino acid sequence of AkChi. We used RT-PCR to evaluate the expression of AkChi in various tissues of A. kurodai, and we observed that AkChi was expressed only in the ovotestis. A phylogenetic tree analysis, performed using the amino acid sequences of AkChi and known GH family 18 chitinases, showed that AkChi was separated from the molluscan chitinases with a chitin binding domain. To our knowledge, this is the first study demonstrating the cDNA cloning of an ovotestis chitinase from a sea hare.

红宝石梨园土壤微生物群落与养分对低分子有机酸的响应

【目的】从梨土壤养分与微生物群落方面,探究红宝石梨树土壤养分与微生物群落应对低分子有机酸的变化规律,并分析梨树土壤微生物群落与养分吸收及果实品质之间的关系。【方法】以施用氮磷钾肥为对照,设置5%与10%的苹果酸(LM与HM)、柠檬酸(LC与HC)、草酸(LO与HO)与氮磷钾肥配施为处理,测定梨树土壤养分与微生物群落功能多样性等指标。【结果】与对照相比,低分子有机酸处理降低了梨园土壤EC值,柠檬酸与草酸显著降低了梨园土壤pH,而柠檬酸与LO处理显著降低了有机质含量。LC显著降低了土壤硝态氮含量,而LO则显著升高了土壤铵态氮含量。与对照相比,低分子有机酸显著降低了0~20 cm土层土壤有效P含量,而LM显著升高>20~40 cm土层速效K含量。另外,低分子有机酸显著改变了梨树土壤微生物群落多样性指数与碳源利用特征,其中HM显著升高0~20 cm土层多样性指数,而LO则显著降低了羧酸类与氨基酸类的利用强度。相关分析表明,0~20 cm土层微生物群落与果实维生素C含量、果实氮磷钾含量、产量等呈负显著相关,而>20~40 cm土层微生物群落与单果质量、果实色泽、果实钾含量以及叶片氮含量呈正显著相关。【结论】苹果酸、柠檬酸及草酸与氮磷钾配施改变了梨园土壤养分含量与微生物群落碳特征,与0~20 cm土层相比,>20~40 cm土层微生物群落在梨树养分吸收与果实品质提升方面发挥着更为重要的作用。

基于叶绿体DNA条形码的披麻草药材及其混伪品的分子鉴定

目的:分析trnV-atpE、psaC-ndhE序列变异特点,并通过该序列鉴别披麻草不同基原植物与其混伪品。方法:分别提取披麻草3种基原植物及其混伪品的总DNA,以trnV-atpE、psaC-ndhE为DNA条形码候选序列进行聚合酶链式反应(PCR)扩增和测序。采用DnaSP、MEGA软件统计其片段长度、鸟嘌呤(G)+胞嘧啶(C)占比、变异位点个数、简约信息位点、插入或缺失位点,并计算样品K2-P(Kimura 2-parameter)遗传距离和构建邻接法(NJ)系统发育树。结果:trnV-atpE、psaC-ndhE序列长度分别为373~381、491~534 bp,简约信息位点分别为18、15个。trnV-atpE和psaC-ndhE序列中披麻草3种基原植物最大遗传距离均小于与混伪品之间的最小遗传距离。基于2个序列构建的NJ系统发育树显示,披麻草与其混伪品能明显区分。结论:综合分析序列特点和种内、种间变异性,trnV-atpE和psaC-ndhE序列均可将披麻草3种基原植物与其混伪品区分开。

艳锦竹芋叶斑病病原菌的分离与鉴定

明确在福建省武夷山市艳锦竹芋上发现的叶斑病病原菌,以期为该病害的防控提供参考。2021年采集武夷学院园艺大棚内患叶斑病的艳锦竹芋(Stromanthe sanguinea‘Triostar’)叶片,通过传统微生物培养方法分离纯化病原菌,并按照科赫氏法则测定其致病性,并对其进行形态学鉴定和基于ITS序列的分子鉴定,并通过系统发育树的构建,分析其遗传多样性。结果表明:从病叶中分离得到病原菌(标记为YJ-2),具有致病性,且与田间发病症状一致。基于ITS序列进行PCR扩增和测序,序列表明菌株YJ-2和NCBI核酸数据库中拟茎点霉属菌Phomopsis sp.(登录号DQ780431.1)的相似性为99.43%,且在系统发育树上聚在一起。根据形态特征和分子鉴定结果,将该地区艳锦竹芋叶斑病病原菌鉴定为拟茎点霉属菌,为国内首次报道拟茎点霉属菌引起的艳锦竹芋叶斑病。

不同地域来源牡丹的亲缘关系分析

【目的】探究西南牡丹品种群与不同种源牡丹品种的亲缘关系,为其栽培起源研究提供基础资料。【方法】以50个中原牡丹品种、20个西南牡丹品种、18个西北牡丹品种、6个国外牡丹品种、1个江南牡丹品种和2个野生种共计96份不同地理种源牡丹为材料,利用36个目标起始密码子多态性(start codon targeted polymorphism,SCoT)引物进行PCR扩增,筛选多态性比率好的条带,利用NTSYS-pc软件计算品种间的遗传相似性系数,在此基础上,采用UPGMA聚类分析个体间的亲缘关系。【结果】多态性好的引物共有18个,用其对96个牡丹样本进行扩增,共获得182条扩增条带,其中多态性条带172个,多态性比率为94.50%;96个样本间的遗传相似性系数在0.5523~0.8681,品种间遗传差异较大,其中遗传相似性系数最大的是西北牡丹品种2与品种3,而紫斑牡丹与豆绿和中甸紫2的遗传相似性系数最小。在遗传相似性系数为0.6931时,96个牡丹样本聚为8支,第1支由15个中原牡丹品种、4个西南牡丹品种和1个江南品种组成;第2支由2个西南牡丹品种丽江紫3和昭通粉1组成;第3支由35个中原传统牡丹品种聚成;第4支包括3个日本品种、1个法国品种和14个西南品种;第5支由17个紫斑牡丹杂交品种聚成;第6支仅有紫斑牡丹1个样本;第7支仅有黄牡丹1个样本;第8支由美国品种海黄和法国品种金晃聚成。【结论】西南牡丹品种与日本牡丹关系最近,与中原牡丹也有着近缘关系,而与其他种源的品种群关系较远。产地对西南牡丹品种的亲缘关系影响较大。

饮用水中铜绿假单胞菌全基因组分析与分子溯源

目的:为湖南省饮用水中铜绿假单胞菌的溯源研究和污染防治提供数据支持。方法:按GB 8538—2016检验湖南省部分市县随机采集的桶装水,对分离鉴定的18株铜绿假单胞菌进行全基因组测序、分子溯源以及毒力基因和耐药基因分析。结果:通过系统进化树分析可知,18株铜绿假单胞菌有明显的聚类分布,清晰反映了样本菌株的亲缘远近情况;通过统计分析毒力基因和耐药基因,证实4株铜绿假单胞菌在地域分布、同源性、致病基因和耐药基因型上呈现一致性,推测为同一来源。结论:基于全基因测序、16S rRNA和单拷贝直系同源分析,可实现饮用水中铜绿假单胞菌的溯源、毒力基因及耐药基因分析。