辣椒果胶裂解酶基因家族的生物信息学分析

为了解辣椒果胶裂解酶(Pectin lyase like,PLL)基因家族成员数量、理化结构及可能参与的生物学过程,以期为全面鉴定和认识辣椒CaPLLs基因家族的生物学功能提供研究基础。利用全基因组扫描方法和在线生物信息学工具对辣椒CaPLLs基因家族进行了鉴定和分析。结果在辣椒参考基因组的9条染色体上共鉴定出28个CaPLLs基因家族成员,且分别隶属于5个亚族;CaPLLs家族成员的氨基酸序列长度介于183~762 aa,分子量范围为19.65~84.31 kDa,等电点范围为5.39~9.44。保守基序及结构域分析表明,CaPLLs家族成员共有10个保守基序,所有成员均含有Pec_lyase_C结构域。有多种与激素、胁迫应答和生长发育相关的顺式作用元件存在于CaPLLs基因的启动子区域中。由此可见,这28个CaPLLs基因家族成员同一亚家族基因之间高度保守。

自噬相关基因ARHⅠ和DAPK在皮肤鳞癌中的表达及意义

目的探讨Ras同源基因家庭成员Ⅰ(ARHⅠ)、死亡相关蛋白激酶(DAPK)在皮肤鳞癌中的表达及意义。方法通过免疫组化法检测正常皮肤组织、Bowen病组织、皮肤鳞癌组织中ARHⅠ、DAPK阳性表达情况,通过实时荧光定量聚合酶链式反应检测正常皮肤组织、Bowen病组织、皮肤鳞癌组织中ARHⅠmRNA、DAPK mRNA相对表达量。分析ARHⅠmRNA、DAPK mRNA相对表达量与皮肤鳞癌严重程度的关系。结果正常皮肤组织、Bowen病组织、皮肤鳞癌组织中ARHⅠ、DAPK阳性表达细胞依次减少,Bowen病组织、皮肤鳞癌组织中的ARHⅠ、DAPK阳性表达率低于正常皮肤组织(P<0.05)。Bowen病组织、皮肤鳞癌组织中的ARHⅠmRNA、DAPK mRNA相对表达量少于正常皮肤组织(P<0.05)。随着皮肤鳞癌的加重,ARHⅠmRNA、DAPK mRNA相对表达量降低,其与皮肤鳞癌严重程度均呈负相关(r=-0.940、-0.932,P<0.01)。结论ARHⅠ、DAPK在皮肤鳞癌组织中下调或缺失,可能与皮肤鳞癌的发生、发展有重要关系。

植物基因家族的分子进化

植物基因家族的分子进化曾庆平，郭勇（华南理工大学生物工程系，广州５１０６４１）关键词基因家族，同源性，分子进化，生物工程建立基因数据库与计算机检索程序使不同基因之间的碱基序列同源性的比较成为可能，同时也有助于进行基因的分子起源与进化以及蛋白质结构与功...

RASSF1A基因甲基化与肝细胞癌关系的Meta分析

目的探讨RAS相关结构家庭1A基因（RASSF1A基因）异常甲基化与肝细胞癌的关系。方法检索国外Pub Med、Embase、Ovid、Web of science、Cochrane Library数据库和国内的中国生物医学文献数据库（CBM）、中文科技期刊全文数据库（VIP）、中国期刊全文数据库（CNKI）、万方数据库2014年7月以前的相关文献,按纳入排除标准筛选文献并提取数据。用Rev Man5.2软件进行统计分析,使用比值比（OR）及95%置信区间（95%CI）衡量RASSF1A基因启动子区甲基化与肝癌的关系。结果共15篇文献1 417例患者纳入研究,其中肝细胞癌组710例、对照组707例。肝细胞癌组织中RASSF1A甲基化阳性率高于正常肝组织[OR=50.23,95%CI（22.21~113.61）、P〈0.05]、癌旁正常组织[OR=7.63,95%CI（3.38~17.22）,P〈0.05]及肝硬化组织[OR=17.18,95%CI（2.57~114.91）,P〈0.05]。结论RASSF1A基因的高甲基化导致该基因的失活,与肝细胞癌的发生发展密切相关。

夹脊电针刺激通过PKA/RhoA通路治疗大鼠急性脊髓损伤

目的:探究电针(EA)夹脊穴对脊髓损伤(SCI)大鼠后肢运动功能及蛋白激酶A(PKA)/Ras同源基因家族成员A(RhoA)通路表达的影响,并从PKA/RhoA通路初步探讨其机制。方法:将36只雌性SD大鼠随机分为假手术组(Sham)、SCI模型组(SCI)、电针干预组(SCI+EA)。运用钳夹法建立SCI模型,SCI+EA组电针干预T_(9)和T_(11)两对夹脊穴。利用脊髓功能评分(BBB量表)检测大鼠的后肢运动功能,HE染色观察脊髓组织形态学改变,同时运用免疫荧光染色、Western Blot及real time RT-PCR检测脊髓组织中蛋白激酶A(PKA)、Ras同源基因家族成员A(RhoA)及生长相关蛋白-43(GAP-43)的表达。结果:SCI模型大鼠后肢运动功能发生严重障碍,脊髓组织结构紊乱,伴较多出血点,而电针刺激后SCI大鼠脊髓组织结构较完整,出血点减少,后肢运动功能也得到明显改善。此外,夹脊电针刺激可显著提高SCI大鼠脊髓组织中PKA mRNA表达,(P<0.05)。同时,夹脊电针刺激后SCI大鼠脊髓组织中PKA、GAP-43蛋白以及磷酸化蛋白p-RhoA(ser188)表达均显著升高(P<0.05)。结论:夹脊电针能改善SCI大鼠后肢运动功能,减轻脊髓组织的病理学损伤;可能是通过调节PKA/RhoA信号通路实现的。

腺病毒介导的RNAi对VaD大鼠脑内NgR/RhoA/ROCK2信号通路的影响

目的探讨基于腺相关病毒为载体构建的Nogo受体(NgR)抑制剂通过NgR/Ras基因家族成员(Rho)A/Rho相关激酶(ROCK)2信号通路改善血管性痴呆(VaD)大鼠学习记忆能力及轴突再生分子机制。方法将40只SD大鼠随机分为假手术组、模型组、NgR干扰剂组(腺相关病毒)、阴性对照组(NgR空载体病毒),每组10只。采用双侧颈总动脉永久结扎术法制作VaD大鼠模型,模型成功后,将AAV9-NgR-shRNA通过脑立体定位术注射至大鼠海马组织,阴性对照组注入等量空载体腺相关病毒。4 w后,采用Morris水迷宫测定学习、记忆能力,采用实时荧光定量-聚合酶链反应(PCR)、Western印迹检测各组NgR/RhoA/ROCK2通路NgR、RhoA、ROCK2 mRNA及蛋白表达水平,电镜观察大鼠海马突触超微结构变化。结果术后1 w,模型组、阴性对照组潜伏期时间与跨越平台次数与NgR干扰组比较,差异无统计学意义(P>0.05),与假手术组比较有显著性差异(均P<0.05)。术后4 w,与模型组及阴性对照组比较,NgR干扰组潜伏期显著缩短,跨越平台次数显著增加,海马中NgR、RhoA、ROCK2 mRNA及其蛋白表达显著减少(均P<0.05),且海马组织内突触前后囊泡正常、细胞器更加完整;阴性对照组上述指标与模型组比较差异无统计学意义(均P>0.05)。结论NgR抑制剂可能通过抑制NgR/RhoA/ROCK2信号通路起到促进神经轴突再生,改善海马突触结构,减轻VaD大鼠认知功能障碍的作用。

水稻野败型细胞质雄性不育系统花药的RRM特异引物差异展示分析

根据 RRM RNA结合蛋白基因家族共有保守序列设计特异引物 ,对水稻野败型细胞质雄性不育系、保持系、恢复系及 F1杂种单核期花药进行差异展示分析。不同材料间具有稳定表达的组成型RRM RNA结合蛋白基因 ,同时具有丰富的差异表达的具调控功能的 RRM RNA结合蛋白基因。不同材料间差异表达的 RRM RNA结合蛋白基因类型分析说明 RRM RNA结合蛋白基因家族参与了细胞质雄性不育系统的核质互作。

肝癌组织FAM96B表达变化及其意义

目的观察肝癌组织96序列相似家庭成员B(FAM96B)mRNA和蛋白表达变化,并探讨其临床意义。方法选择42例肝癌患者,采用实时荧光定量PCR法检测肝癌组织及癌旁正常肝组织中FAM96B mRNA表达,采用Western blotting法检测FAM96B蛋白表达,并分析肝癌组织FAM96B蛋白表达与患者临床病理参数的关系。结果肝癌组织和癌旁正常肝组织FAM96B mRNA相对表达量分别为0.423±0.096、1.649±0.268,FAM96B蛋白相对表达量分别为0.845±0.131、1.548±0.234。肝癌组织和癌旁正常肝组织FAM96B mRNA和蛋白相对表达量比较,P均<0.05。肝癌组织FAM96B蛋白相对表达量与肝癌大小、门静脉癌栓、肝外转移、Child分级、BCLC分期有关(P均<0.05),与患者性别、年龄、肿瘤数目、乙肝、肝硬化、血清AFP无关(P均>0.05)。结论肝癌组织FAM96B mRNA和蛋白表达降低。检测肝癌组织FAM96B蛋白表达量有助于判断患者病情。

吡哆醇依赖性癫痫的临床及乙醛脱氢酶7家庭成员A1基因突变分析

目的分析1例吡哆醇依赖性癫痫（PDE）的临床诊治过程及乙醛脱氢酶7家庭成员A1（ALDH7A1）基因突变特征。方法对1例以早期癫痫起病的PDE患儿行临床诊治观察、神经电生理及神经影像学检查、以及ALDH7A1基因突变分析。结果患儿出生2个月出现反复癫痫发作，多种抗癫痫药均不能控制发作，多次住院过程中在抗癫痫药治疗基础上给予吡哆醇静脉滴注使发作控制，出院后仅用抗癫痫药而未用吡哆醇维持治疗，癫痫发作分别在吡哆醇撤药后13d、14d及38d出现复发，减停抗癫痫药物后仅单纯口服吡哆醇使发作完全控制。治疗前后多次EEG正常，头颅MRI检查正常。ALDH7A1基因检测发现1对新的复合杂合突变，第5外显子c．410G〉A（P．G137E）和第11内含子IVS11＋1G〉A剪切位点突变，其父携带G137E突变，其母携带IVSll＋1G〉A突变。结论本例癫痫发作早期起病、经吡哆醇治疗有效、撤药后复发临床提示了PDE的可能，ALDH7A1基因分析最终确诊了国内第1例PDE，本例携带的2个基因突变位点均为国际未报道的新位点。

沈阳地区家庭聚集性感染HBV的家庭HBV前C区基因突变率及其临床意义的研究

目的 研究沈阳地区家庭聚集性感染乙型肝炎病毒的家庭HBV前C区 1896位G→A基因突变率及其临床意义。方法 采用PCR RFLP法检测HBV前C区 1896位G→A基因突变。结果 患者及其家庭成员HBV前C区 1896位G→A基因突变发生率分别为 5 6 .3%和 4 0 .5 % ,明显高于患者配偶 2 5 0 %的突变发生率 ,且配偶中抗 HBs阳性率为 2 6 .3%。同时 ,这种突变在慢性乙型肝炎患者中的发生率为 5 2 .4 % ,在HBV携带者中的发生率为 4 4 .4 % ,在慢性重型肝炎患者中的发生率仅为 2 0 0 %。结论 HBV前C区 1896位G→A基因突变的发生 ,可能与HBV的持续感染有关。

Expressions of genes related to genome stability and DNA repair in nasopharyngeal carcinoma clustering families

Objective： The aim of the study was to observe the expressions of genes related to genome stability and DNA repair in the members of nasopharyngeal carcinoma （NPC） clustedng families. Methods： In the Zhongshan City where there is highly incidence rate of NPC, we chose the members of the NPC clustering families as objects, and the patients of nasopharyngitis and NPC as the control group. We isolated the RNA from the nasopharyngeal tissue, and synthesized its cRNA, the genome stability and DNA repair genes chip technique, chemiluminescent detection and real-time fluorescence quantita- tive technique were used to examine the genome stability and DNA repair genes in the nasopharyngeal tissue. Results： More genome stability and DNA repair genes were up-regulated in the members of the NPC clustering families than the NPC patients, and the range of up-regulated was high, with the over up-regulated 100 times genes including TEP1, MSH4, PMS2LI. Fewer genome stability and DNA repair genes were down-regulated in the members of the NPC clustering families than the NPC patients, the ubiquitin genes almost were down-regulated, the results also could be confirmed by real-time fluorescence quantitative PCR. Conclusion： There are specially expression character of genome stability and DNA repair genes in the members of NPC clustering families.

Evidence from a familial case suggests maternal inheritance of primary biliary cholangitis

Primary biliary cholangitis(PBC) is an idiopathic autoimmune liver disease characterized by chronic cholestasis and destruction of the intrahepatic bile ducts. Similar to other autoimmune diseases, the pathogenesis of PBC is considered to be a complex etiologic phenomenon involving the interaction of genetic and environmental factors. Although a number of common variants associated with PBC have been reported from genome-wide association studies, a precise genetic mechanism underlying PBC has yet to be identified. Here, we describe a family with four sisters who were diagnosed with PBC. After the diagnosis of the index patient who was in an advanced stage of PBC, one sister presented with acute hepatitis, and two sisters were subsequently diagnosed with PBC. Notably, one half-sister with a different mother exhibited no evidence of PBC following clinical investigation. Our report suggests the possibility of a maternal inheritance of PBC susceptibility. Moreover, judging from the highpenetrance of the disease observed in this family, we inferred that a pathogenic genetic variant might be the cause of PBC development. We describe a family that exhibited diverse clinical presentations of PBC that included asymptomatic stages with mildly increased liver enzyme levels and symptomatic stages with acute hepatitis or advanced liver fibrosis. Additional studies are needed to investigate the role of genetic factors in the pathogenesis of this rare autoimmune disease.

Attenuated adenomatous polyposis of the large bowel: Present and future

Attenuated adenomatous polyposis(AAP) is a poorly understood syndrome, that can be defined as the presence of 10-99 synchronous adenomas in the large bowel, and it is considered a phenotypic variant of familial adenomatous polyposis(FAP). This definition has the advantage of simplicity, but it may include sporadic multiple adenomas of the large bowel at an extreme, or FAP cases on the other side. AAP shows a milder phenotype than FAP, with an older age of onset of adenomas and cancer, and less frequent extracolonic manifestations. AAP may be diagnosed as a single case in a family or, less frequently, it may be present in other family members, and it shows distinct pattern of inheritance. In less than 50% of cases, it may be caused by adenomatous polyposis coli(APC) or MUTYH mutations, referred to as APC-associated polyposis, inherited as an autosomal dominant trait, or MUTYH-associated polyposis, which shows an autosomal recessive mechanism of inheritance, respectively. Surveillance should rely on colonoscopy at regular intervals, with removal of adenomas and careful histological examination. When removal of polyps is not possible or advanced lesions are observed, the surgical approach is mandatory, being subtotal colectomy with ileo-rectal anastomosis the treatment of choice. Studies on this syndrome are lacking, and controversies are still present on many issues, thus, other clinical and genetic studies are requested.

Genetically confirmed familial hypercholesterolemia in outpatients with hypercholesterolemia

Background Familial hypercholesterolemia （FH） is an autosomal dominant disorder of lipoprotein metabolism which can lead to premature coronary heart disease （pCHD）. There are about 3.8 million potential FH patients in China, whereas the clinical and genetic data of FH are limited. Methods Dutch Lipid Clinic Network （DLCN） criteria was used to diagnose FH in outpatients with hypercholesterolemia. Resequencing chip analysis combined with Sanger sequencing validation were used to identify mutations in the definite FH patients according to DLCN criteria. In silico analysis was conducted in mutations with previously unknown pathogenicity. Then, the novel mutant receptors were transfected into human embryo kidney 293 （HEK-293） cells. The binding and the internalization activities of the mu- tant receptors were analyzed by flow cytometry. Results The prevalence of definite FH in outpatients with hypercholesterolemia in this study is 3.2%. Using genetic testing, one homozygous FH （HoFH）, one heterozygous FH （HeFH） and three compound heterozygous FH patients were confirmed. Eight mutations in low-density lipoprotein receptor （LDLR） gene were identified, in which c.357delG was a novel mutation and co-segregated with the FH phenotype. Bioinformatic analysis confirmed that c.357delG was a pathogenic mutation. Furthermore, when compared with the wild-type LDLRs by flow eytometry analysis, the binding and internalization activities of c.357delG mutant LDLRs were reduced by 35% and 49%, respectively. Conclusions This study identified eight LDLR gene mutations in five patients with definite FH, in which c.357delG is a novel pathogenic mutation. These findings increase our understanding of the genetic spectrum of FH in China.

Molecular phylogeny of oligotrich genera Omegastrombidium and Novistrombidium(Protozoa,Ciliophora) for the systematical relationships within Family Strombidiidae

The phylogeny of the oligotrich ciliates is currently a hot debate despite the availability of both morphological and molecular data.In the present paper,further small subunit rRNA(SS rRNA) genes were analyzed from the Genera Omegastrombidium and Novistrombidium,as well as from Strombidium,and combined with three new SS rRNA sequences from Strombidium basimorphum,S.sulcatum population QD-1,and Novistrombidium testaceum population GD.The phylogenetic positions of these organisms were inferred using Bayesian inference,Maximum Likelihood,and Maximum Parsimony methods.The main results are:(1) the SS rRNA gene sequence analyses match the recent findings about the molecular evolution of oligotrichs,indicating that the family Strombidiidae is paraphyletic;(2) the Genus Omegastrombidium is separated from the Genus Strombidium,as shown in recent cladistic analyses;(3) morphospecies in Genus Novistrombidium,based on similarity of somatic ciliature,are separated from each other in all topological trees,indicating that this genus could be a paraphyletic group;(4) the molecular data indicate a possibility of paraphyly for the genus Strombidium;and(5) the similarities of the SS rRNA gene of specimens identified as S.sulcatum and S.inclinatum are 99.8%-100%.However,present knowledge on the oligotrichs sensu stricto is still insufficient and further studies based on both molecular and other technologies are required.

Bilateral Pheochromocytoma as First Presentation of von Hippel-Lindau Disease in a Chinese Family

Objective To investigate the clinical and genetic features of a Chinese family with yon Hippel- Lindau （VHL） disease revealed by bilateral pheochromocytoma. Methods The proband and other members in a Chinese family with familial pheochromocytoma were clinically evaluated and followed up. Genomic DNA extracted from the peripheral blood of 8 family members （including 3 patients） was amplified by polymerase chain reaction （PCR） and the PCR products were directly sequenced. Results The first presentation in the proband, his mother, and his sister was bilateral pheochromocytoma, and the missense mutation of 695G-A （Arg161Gln） in exon 3 of VHL gene was detected in the three patients. In the follow-up study, the proband and his mother were found to have other VHL tumors, induding retinal and cerebellar hemangioblastomas and pancreatic tumor. Neither clinical presentation of VHL disease nor gene mutation was found in other family members. Conclusion VHL disease should be suspected in some patients with familial pheochromocytoma, and VHL gene screening helps to achieve early diagnosis of the disease.

益母草碱对原发性肾病综合征大鼠的影响

目的研究益母草碱(LEO)调节Ras同源基因家庭成员A(RhoA)/Rho相关卷曲螺旋形成的蛋白激酶(ROCK)信号通路对原发性肾病综合征(PNS)大鼠的改善作用。方法培养大鼠肾小球系膜细胞HBZY-1,随机分为对照组、增生组[100 ng·mL^(-1)脂多糖(LPS)]、低浓度实验组(100 ng·mL^(-1)LPS+5μmol·L^(-1)LEO)、高浓度实验组(100 ng·mL^(-1)LPS+10μmol·L^(-1)LEO)和联合处理组(100 ng·mL^(-1)LPS+10μmol·L^(-1)LEO+10 nmol·L^(-1)RhoA激活药U46619)。以细胞计数试剂盒法检测细胞增殖活性,用流式细胞仪检测细胞凋亡情况。将60只SPF级Wistar大鼠随机分为正常组、模型组、低剂量实验组(10 mg·kg^(-1)LEO)、高剂量实验组(20 mg·kg^(-1)LEO)和联合组(20 mg·kg^(-1)LEO+10 mmol·L^(-1)U46619),每组12只。用考马斯亮蓝法检测大鼠24 h尿蛋白含量,用酶联免疫吸附测定法检测大鼠肾组织中炎性因子肿瘤坏死因子-α(TNF-α)、白细胞介素(IL)-4水平,用蛋白质印迹法检测大鼠肾组织RhoA和ROCK1蛋白的表达水平。结果在细胞实验中,对照组和增生组的HBZY-1细胞增殖活性(光密度值)分别为0.32±0.03和0.70±0.07,细胞凋亡率分别为(9.23±1.04)%和(1.64±0.22)%,在统计学上差异均有统计学意义(均P<0.05)。在动物实验中,正常组、模型组、低剂量实验组、高剂量实验组和联合组的24 h尿蛋白含量分别为(21.45±2.28)、(127.38±14.70)、(120.85±13.34)、(43.15±6.68)和(96.20±10.63)mg,TNF-α水平分别为(0.27±0.05)、(1.58±0.16)、(1.56±0.16)、(0.44±0.05)和(1.03±0.10)ng·mL^(-1),IL-4水平分别为(0.17±0.02)、(1.24±0.12)、(1.20±0.12)、(0.29±0.03)和(0.87±0.09)ng·mL^(-1),RhoA蛋白相对表达水平分别为0.27±0.03、0.78±0.08、0.76±0.07、0.34±0.03和0.72±0.07,ROCK1蛋白相对表达水平分别为0.22±0.02、0.85±0.09、0.83±0.08、0.41±0.04和0.75±0.08,联合组的上述指标与高剂量实验组比较,在统计学上差异均有统计学意义(均P<0.05)。结论LEO可能通过下调RhoA/ROCK信号通路对大鼠PNS起到改善作用。

96序列相似的家庭成员B在肝癌中的表达变化及功能研究

目的 探讨96序列相似的家庭成员B（FAM96B）在肝细胞肝癌中的表达,以及对人肝癌细胞株HepG2增殖和凋亡的影响。方法 分别采用实时荧光定量聚合酶链反应（FQ-PCR）及Western blot技术检测FAM96B在42例肝癌肿瘤组织和癌旁组织、HepG2和L-02细胞中的mRNA及蛋白表达量,比较其差异。构建pcDNA3.1-myc-FAM96B真核表达载体,并通过脂质体质粒转染HepG2细胞,采用噻唑蓝（MTT）法及流式细胞仪（FACS）检测FAM96B基因对HepG2增殖及凋亡的影响。结果 42例肝癌组织中,Real-time PCR结果显示FAM96B在肿瘤组织中的mRNA表达量是癌旁组织的（0.304±0.094）倍,且其在HepG2细胞中的mRNA表达量是L-02细胞的（0.406±0.115）倍,差异有统计学意义（P〈0.05）。Western blot结果显示FAM96B在肿瘤组织中的蛋白表达是癌旁组织的（0.288±0.132）倍（P〈0.05）,且其在HepG2细胞中的蛋白表达是L-02细胞的（0.359±0.143）倍（P〈0.05）。MTT细胞实验结果显示FAM96B组吸光度值显著低于对照组（P〈0.05）,即过表达FAM96B可抑制HepG2细胞增殖。流式检测显示过表达FAM96B组的HepG2细胞凋亡率（33.3%）与对照组（3.3%）比较增高,差异有统计学意义（P〈0.05）。结论 FAM96B在42例肝癌肿瘤组织中的表达显著低于癌旁组织,并且其在HepG2细胞中的表达低于L-02细胞,过表达FAM96B可抑制HepG2细胞增殖并诱导其凋亡。该基因可能在肝细胞肝癌的发生发展中发挥重要作用。

A novel deletion mutation of ATP7A gene in a Chinese family with Menkes disease

Menkes disease is a rare X-linked recessive .hereditary disorder first described by Menkes et al in 1962.1 including The gene mutation results in clinical features pili torti, unusual facies, mental/growth retardation and metabolic dysfunction. The pathogenic gene ATP7A was identified in 1993.2 It is located on chromosome X and encodes a transmembrane Cu^2＋ transporter. Here we reported the clinical manifestations and results of genetic study of a family with Menkes disease. In this family, a deletion mutation in ATP7A gene is responsible for the disease.

Genome-wide identification and characterization of phospholipase C gene family in cotton (Gossypium spp.)

Phospholipase C (PLC) are important regulatory enzymes involved in several lipid and Ca2+-dependent signaling pathways.Previous studies have elucidated the versatile roles of PLC genes in growth, development and stress responses of many plants, however, the systematic analyses of PLC genes in the important fiber-producing plant, cotton, are still deficient. In this study,through genome-wide survey, we identified twelve phosphatidylinositol-specific PLC (PI-PLC) and nine non-specific PLC (NPC) genes in the allotetraploid upland cotton Gossypium hirsutum and nine PI-PLC and six NPC genes in two diploid cotton G. arboretum and G.raimondii, respectively. The PI-PLC and NPC genes of G. hirsutum showed close phylogenetic relationship with their homologous genes in the diploid cottons and Arabidopsis. Segmental and tandem duplication contributed greatly to the formation of the gene family. Expression profiling indicated that few of the PLC genes are constitutely expressed, whereas most of the PLC genes are preferentially expressed in specific tissues and abiotic stress conditions. Promoter analyses further implied that the expression of these PLC genes might be regulated by MYB transcription factors and different phytohormones.These results not only suggest an important role of phospholipase C members in cotton plant development and abiotic stress response but also provide good candidate targets for future molecular breeding of superior cotton cultivars.