Effects of Heterologously Overexpressing PIP5K-Family Genes in Arabidopsis on Inflorescence Development

Castor is one of the top 10 oil crops in the world and has extremely valuable uses.Castor inflorescences directly affect yield,so the study of inflorescence development is very important in increasing castor yield.Our previous studies have shown that the PIP5K gene family(PIP5Ks)is associated with inflorescence development.In this study,to determine the function of each PIP5K gene in castor,a female Lm-type castor line,aLmAB2,was used to determine the relative expression levels of the PIP5Ks in castor inflorescences.Six PIP5K genes were heterologously overexpressed in Arabidopsis thaliana,the relative expression of each gene and the effect on plants was determined in A.thaliana,and the relationships among the PIP5Ks in castor were inferred.The expression levels of the PIP5Ks in the female Lm-type castor line aLmAB2 were analyzed.The relative expression levels of the PIP5K9 and PIP5K11 genes were high(p<0.05)in isofemale inflorescences,and those of PIP5K1,PIP5K2,PIP5K6,and PIP5K8 were high(p<0.05)in female inflorescences but low(p<0.05)in bisexual inflorescences.The PIP5Ks were heterologously overexpressed in A.thaliana,and T3-generation plants with stable genetic resistance,i.e.,AT-PIP5K^(+)plants(AT-PIP5K1^(+),AT-PIP5K2^(+),AT-PIP5K6^(+),AT-PIP5K8^(+),AT-PIP5K9^(+),and ATPIP5K11^(+) plants),were obtained.Biological tests of the AT-PIP5K+plants showed that the growth of the main stem was significantly delayed in AT-PIP5K+plants compared with Columbia wild-type(WT)A.thaliana plants;the PIP5K1 and PIP5K2 genes promoted lateral stem growth and flower and silique development;and the PIP5K6,PIP5K8,PIP5K9 and PIP5K11 genes inhibited lateral stem growth and flower and silique development.The correlations among PIP5Ks in castor suggest that there may be a synergistic relationship among PIP5K1,PIP5K2,and PIP5K6 in castor inflorescences,and PIP5K8,PIP5K9,and PIP5K11 are complementary to the other three genes.

Association between 5-HTR1A gene C-1019G polymorphism and antidepressant response in patients with major depressive disorder:A meta-analysis

BACKGROUND Major depressive disorder(MDD)is a substantial global health concern,and its treatment is complicated by the variability in individual response to antide-pressants.AIM To consolidate research and clarify the impact of genetic variation on MDD treatment outcomes.METHODS Adhering to Preferred Reporting Items for Systematic Reviews and Meta-Analyses guidelines,a systematic search across PubMed,EMBASE,Web of Science,and the Cochrane Library was conducted without date restrictions,utilizing key terms related to MDD,serotonin 1A receptor polymorphism(5-HTR1A),C-1019G polymorphism,and antidepressant response.Studies meeting inclusion criteria were thoroughly screened,and quality assessed using the Newcastle-Ottawa Scale.Statistical analyses,includingχ2 and I²values,were used to evaluate heterogeneity and fixed-effect or random-effect models were applied accordingly.RESULTS The initial search yielded 1216 articles,with 11 studies meeting criteria for inclusion.Analysis of various genetic models showed no significant association between the 5-HTR1A C-1019G polymorphism and antidepressant efficacy.The heterogeneity was low to moderate,and no publication bias was detected through funnel plot symmetry and Egger's and Begg's tests.CONCLUSION This meta-analysis does not support a significant association between the 5-HTR1A C-1019G polymorphism and the efficacy of antidepressant treatment in MDD.The findings call for further research with larger cohorts to substantiate these results and enhance the understanding of antidepressant pharmacogenetics.

人Tum-5基因逆转录病毒载体及包装细胞株的构建

目的构建携带Tum-5基因的逆转录病毒载体并对其进行包装,获得稳定的产毒细胞系。方法采用RT-PCR法从胎肾组织中扩增Tum-5基因片断,并将其定向克隆到逆转录病毒载体pLXSN中进行PCR、双酶切和测序鉴定。利用电穿孔方法将获得的重组质粒转染PA317细胞,经G418筛选抗性克隆,收集病毒上清后感染NIH3T3细胞测定病毒滴度。结果PCR、酶切证实Tum-5基因克隆至逆转录病毒载体pLXSN,Tum-5基因测序结果和原始序列相同。重组逆转录病毒载体转染PA317包装细胞,RT-PCR证实转染后的PA317细胞上清液中存在携带人Tum-5基因的病毒RNA,病毒滴度为2.05×104cfu/m。l结论成功的构建了携带人Tum-5基因的逆转录病毒载体,获得了稳定的产毒细胞系。

Rapid Constructing a Genetic Linkage Map by AFLP Technique and Mapping a New Gene tms5

In this study, we reported the repaid construction of a molecular marker linkage map of rice (Oryza sativa L.). An F-2 population from the cross between Annong S-1 and Nanjing 11 was used to construct a genetic linkage map of rice. Total of 142 newly screened AFLP markers and 30 anchor markers (25 SSR markers and 5 RFLP markers) were mapped on the 12 chromosomes covering 1537.4 cM of rice genome. The average interval between these markers was 9.0 cM. The total work which usually was finished in more than one year was finished within only 3 months by one person. This is the first plant AFLP map developed in China. A new thermosensitive genic male sterile gene in rice, tms5, was Egged and mapped onto chromosome 2 during the development of the linkage map.

Analysis on Heredity and Variation of the ORF_5 Gene of Prevalence Strains Porcine Reproductive and Respiratory Syndrome Virus

[ Objective] The aim was to analyze the reason and epidemic trend of PRRSV, and provide theoretical basis for preventing and controlling PRRS. [Methed]According to the sequence of ATCC VR-2332 strain porcine reproductive and respiratory syndrome virus published by the GenBank, the primers were designed and synthesized. ORF5 gene sequences of seven prevalence strains were amplified by RT-PCR. The sequences of ORF5 genes were analyzed by DNAStar and compared with those of ATCC VR-2332, CH-1 a, B J-4, LV-M96262 and MLV vaccine strains, phylogenetic tree among isolates was analyzed. [Result] Analysis of nucleotide sequence showed that the homology was 88.1% - 98.8%, 89.9% -95.2%, 85.6% -98.7% between ORF5 genes of seven prevalence strains and VR-2332, CH-1a, BJ-4, and the homology was 54.7% -56.9% between ORF5 genes and LV. Analysis of amino acid sequence showed that the homology was 88.1% -96.8%, 88.1% - 94.5%, 86.1% -96.5% between ORF5 genes of seven prevalence strains and VR-2332, CH-1a, bBJ-4, the homology was 54.7% -56.2% between the ORF5 genes and LV.[ Conclusion] The variation of prevalence strains was great in the ORF5 gene region, the homology of ORF5 gene sequence was higher and genetic relationship was nearer during prevalence strains in the same region, or was far in different regions.

重组人Tum-5融合蛋白的克隆、表达、纯化及鉴定

目的:构建人肿瘤抑素(tumstatin)活性片段Tum5的融合重组表达载体并对其进行诱导表达和蛋白纯化以获得大量重组融合蛋白.方法:人工合成Tum5基因,进行测序分析,将该基因克隆入原核表达载体pQE30中,转化感受态细胞DH5α,经IPTG诱导表达重组融合蛋白,对表达产物进行TricineSDSPAGE电泳分析和WesternBlot检测分析.结果构建了重组融合表达质粒pQE30Tum5,表达的蛋白经TricineSDSPAGE电泳分析,在约Mr10×103处出现了一条新生的蛋白条带,经灰度扫描检测,表达量约占菌体总蛋白的40%,纯化后的蛋白灰度扫描检测,纯度为95%.结论:成功地构建了人Tum5基因的原核表达载体,并纯化了该基因的原核表达产物.

Genetic Variation of the ORF5 Gene of Porcine Reproductive and Respiratory Syndrome Virus in East China during 2008-2010

[Objective] A total of 260 swine samples of dead or sick pigs collected from 7 provinces （municipalities） Jiangsu, Anhui, Shanghai, Shandong, Zhejiang, Fujian and Jiangxi of China during 2008-2010 were detected for porcine reproductive and respiratory syndrome virus （PRRSV）. And the ORF5 genes of some isolates were amplified and sequenced for understanding the molecule epidemiology and the genetic evolution of PRRSV in East China. [Method] Using RT-PCR method, PRRSV was detected by RT-PCR from samples. The complete ORF5 genes of 36 PRRSV positive samples was amplified, sequenced and analyzed with other 15 strains available on GenBank. [Result] PRRSV was detected in 118/260 of the clinical samples, with a positive rate was 45.4%. Sequence analysis showed that the 36 isolates of this study belonged to the North American-type PRRSV strains and were closely related to the highly pathogenic PRRSV （HP-PRRSV） with 94.6%-100% amino acid sequence identities. The sequence analysis combined with the phylogenetic analysis indicated that all these North American-type PRRSV strains in East China were further divided into five subgenotypes, subgenotype Ⅲ showed closer identity with HPPRRSV; almost all subgenotypes were found to be variable in the primary neutralizing epitope; subgenotypes Ⅲ and IV had more glycosylation sites than others. Although these 36 isolates were collected from different provinces in East China, there were no obvious relations between the distribution of PRRSV and the region. [Conclusion] The PRRSV infection was widespread and HP-PRRSV was the popular strain in East China during 2008-2010. However some different genetic characteristics appeared in the genomes, the genetic evolution was relatively stable. There exists a cross-cutting phenomenon on the genetic relationship of PRRSV isolates obtained from different provinces. Subgenotypes IV and V only appeared in some provinces, but the distribution of PRRSV did not show apparent geographical characteristics.

Tumstatin基因抗肿瘤血管生成片段Tum-5的研究进展

本文就肿瘤抑素(Tumstatin)抗血管生成活性片段Tum-5的相关研究进展做一综述。

小儿脑性瘫痪与ATG5多态性的关联性及危险因素分析

目的分析自噬相关基因5(ATG5)多态性与小儿脑性瘫痪(CP)的关联性,探究影响CP发生的危险因素。方法选择2022年1月—2024年1月我院收治的118例CP患儿为研究对象,纳入研究组;选择同期收治的200例非CP小儿纳入对照组。应用聚合酶链式反应-限制性酶切片段长度多态性(PCR-RFLP)技术检测ATG5基因单核苷酸多态性(SNP)位点rs510432、rs573775、rs2299863、rs3804338、rs6568431多态性,采用酶联免疫吸附试验(ELISA)法检测2组儿童血浆ATG5水平,采用logistic回归分析ATG5基因多态性与小儿CP易感性的关系。结果研究组和对照组ATG5基因rs6568431位点AA、AC、CC基因型频率分别为25.42%、40.68%、33.90%和8.00%、40.00%、52.00%,差异有统计学意义(P<0.05),2组儿童rs510432、rs573775、rs2299863、rs3804338位点各基因型频率比较,差异均无统计学意义(P>0.05)。研究组和对照组儿童ATG5基因rs6568431位点A、C等位基因频率分别为45.76%、54.24%和28.00%、72.00%,差异有统计学意义(P<0.05),rs510432、rs573775、rs2299863、rs3804338位点各等位基因频率比较,差异均无统计学意义(P>0.05)。研究组儿童血浆ATG5水平为(8.42±0.95)ng/mL,明显低于对照组的(10.67±0.99)ng/mL,差异有统计学意义(t=19.872,P<0.05),且携带AA基因型儿童的血浆ATG5水平明显低于携带AC+CC基因型儿童,差异有统计学意义(P<0.05)。单因素分析结果显示,2组儿童母亲既往不良孕产史、母亲妊娠期高血压、母亲孕期羊水异常、宫内窘迫、病理性黄疸以及缺血缺氧性脑病情况的差异均有统计学意义(P<0.05)。多因素logistic回归分析结果显示,母亲有既往不良孕产史、母亲孕期羊水异常、宫内窘迫、病理性黄疸、缺血缺氧性脑病以及ATG5基因rs6568431位点多态性是CP发生的影响因素,差异均有统计学意义(P<0.05)。结论ATG5基因rs6568431位点多态性与小儿CP易感性存在关联性,且携带AA基因型可能增加小儿CP发生风险。此外,小儿CP的发生还与母亲既往不良孕产史、母亲孕期羊水异常、宫内窘迫、病理性黄疸以及缺血缺氧性脑病等多种因素有关,故针对高危因素进行积极预防,有助于减少小儿CP的发生。

血清抗黑色素瘤分化相关基因5阳性皮肌炎胸部CT特征定性及定量分析

目的 定性及定量分析血清抗黑色素瘤分化相关基因5(MDA-5)抗体阳性的皮肌炎患者胸部CT特征及其与短期预后的关系。资料与方法 回顾性纳入2017年1月—2018年12月中日友好医院收治的67例MDA-5阳性的皮肌炎患者,分析胸部CT特征与短期不良预后的关系。结果 9例患者1年内死亡。死亡组与存活组间质性肺疾病(ILD)影像学类型(χ^(2)=9.964,P=0.025)和肺动脉直径/主动脉直径比值(U=103.0,P=0.004)差异有统计学意义。抗MDA-5抗体阳性的皮肌炎患者合并ILD影像学类型主要为机化性肺炎。弥漫性肺泡损伤的患者死亡率显著高于其他几种类型。Logistic回归分析显示,肺动脉直径/主动脉直径比值(OR 4.208,P=0.002)是抗MDA-5抗体阳性的皮肌炎合并ILD患者发生死亡的强独立危险因素。结论 MDA-5阳性皮肌炎患者大部分伴ILD,其中以机化性肺炎为主要特征。1年内不良预后患者ILD类型不同,但肺动脉直径/主动脉直径比值是MDA-5阳性皮肌炎合并ILD患者发生死亡的独立危险因素。

乳腺癌组织miR-1247-5p表达及其靶基因生物信息学预测研究

目的:探讨微小核糖核酸-1247-5p(miR-1247-5p)在乳腺癌组织中的表达,并对其预测的靶基因进行生物信息学分析。方法:收集2019年6月至2020年12月本院手术治疗的104例乳腺癌患者癌组织及其癌旁组织。RT-PCR检测标本中miR-1247-5p的相对表达量;比较不同临床病理特征患者癌组织miR-1247-5p表达;预测miR-1247-5p的靶基因;采用DAVID数据库对miR-1247-5p靶基因进行功能和通路富集分析;String数据库对miR-1247-5p靶基因进行互作分析。结果:miR-1247-5p在乳腺癌组织中的表达水平较癌旁组织下调(P<0.05)。miR-1247-5p潜在靶基因38个,其靶基因功能主要富集于RNA聚合酶Ⅱ启动子的转录调控、基因表达/转录调控、质膜部分、突触小体、蛋白质结合、poly(A)RNA结合等;参与的通路主要富集于癌症通路、细胞因子与细胞因子受体的相互作用、磷脂酰肌醇3激酶(PI3K)-蛋白激酶B(Akt)信号通路等。磷酸酯酶与张力蛋白同源物(PTEN)、上皮生长因子受体(EGFR)、假尿苷酸合酶1(PUS1)的编码蛋白质在miR-1247-5p基因靶基因蛋白质互作网络(PPI)中关键节点位置。结论:miR-1247-5p在乳腺癌组织中的表达下调,其靶基因富集于多个生物学过程及与肿瘤相关的信号转导通路上,miR-1247-5p可能通过调控其靶基因的表达参与乳腺癌的发生发展过程。

抗MDA5抗体阳性幼年皮肌炎临床特点及治疗转归分析

目的分析抗黑色素瘤分化相关基因5(MDA5)抗体阳性幼年皮肌炎(JDM)的临床特点及治疗转归。方法收集首都医科大学附属北京儿童医院风湿科2015年6月至2022年2月收治的487例JDM患儿的临床资料,其中41例(8.42%)为抗MDA5抗体阳性者。对其临床特点、疾病评估、治疗药物及疾病转归进行总结分析。结果41例抗MDA5抗体阳性JDM患儿中,最常见的临床表现是皮肤和黏膜异常,其次为肌无力,发热和关节炎也较为常见,部分患儿出现呼吸系统症状和皮肤溃疡。皮肤评估工具(CAT)评分以3~5分占大多数。儿童肌炎评估量表(CMAS)评分为(33.88±9.57)分。间质性肺疾病(ILD)的发病率为87.80%,12.20%的患儿发展为快速进展型ILD(RP-ILD)。5例(12.20%)在病程中出现皮下钙化。90.24%的抗MDA5抗体阳性JDM患儿有高危病征。静脉注射甲基泼尼松龙(IVMP)(63.41%)、静脉注射免疫球蛋白(IVIG)(68.29%)和口服环孢素A(65.85%)是治疗的主要方法。9例(21.95%)患儿口服托法替布。75.61%的患儿表现为单一病程,19.51%的患儿为复发性病程,4.88%的患儿为持续的活动性病程。1年、2年、3年和4年的完全临床应答率分别为65.79%(25/38)、65.38%(17/26)、63.64%(14/22)和70.59%(12/17)。5年完全临床缓解率为14.29%(2/14),2年疾病复发率为19.23%(5/26)。在2年的随访中,95.00%(19/20)的患儿肺部病变完全吸收。随访3个月、6个月、9个月和12个月时,泼尼松的中位剂量分别为1.40 mg/kg、1.00 mg/kg、0.71 mg/kg和0.60 mg/kg,糖皮质激素停用的中位时间为69个月。截至2022年2月,41例患儿中有15例(36.59%)停用糖皮质激素,9例(21.95%)停用所有药物。结论抗MDA5抗体阳性JDM是一种特殊类型的JDM,主要表现为特征性皮疹、肌无力、发热和关节炎,ILD是主要危害。该病完全临床缓解率仍然较低,复发率相对较高。

表达SFTSV Gn基因的重组5型腺病毒的构建与鉴定

为了构建出表达新布尼亚病毒(SFTSV)Gn基因的重组5型腺病毒,试验根据GenBank上发表的SFTSV Gn基因序列(登录号为ADZ04482.1)设计合成引物,采用特异性PCR方法在Gn基因前添加了KOZAK序列和tPA信号肽序列;然后通过酶切、连接等方法构建重组穿梭质粒PGA-KOZAK-tPA-Gn,与腺病毒骨架质粒pAd5-ΔE1ΔE3-5E4在BJ5183感受态细胞中进行同源重组,得到重组腺病毒质粒rAd5-KOZAK-tPA-Gn,用PacⅠ酶酶切重组腺病毒质粒,并将线性化的质粒转染至HEK 293细胞中进行病毒包装、扩繁和纯化;采用PCR扩增、Western-blot等技术检测病毒基因的表达情况,并测定重组腺病毒效价。结果表明:通过PCR扩增获得了1 546 bp的KOZAK-tPA-Gn基因,并成功构建了重组穿梭质粒;SFTSV Gn基因在重组腺病毒传代过程中稳定存在;重组腺病毒在HEK 293细胞中表达出分子量约为61 ku的SFTSV Gn蛋白;测得重组腺病毒效价为1×10^(-7.63)/0.1 mL TCID_(50)。说明试验成功构建出表达SFTSV Gn基因的重组5型腺病毒。

Possible association of the 5-HTTLPR serotonin transporter promoter gene polymorphism with premature ejaculation in a Turkish population

We evaluated the genotypes of the serotonin transporter gene （5-HTT） in patients with premature ejaculation （PE） to determine the role of genetic factors in the etiopathogenesis of PE and possibly to identify the patient subgroups. A total of 70 PE patients and 70 controls were included in this study. All men were heterosexual, had no other disorders and were either married or in a stable relationship. PE was defined as ejaculation that occurred within 1 min of vaginal intromission. Genomic DNA from patients and controls was analyzed using polymerase chain reaction, and allelic variations of the promoter region of the serotonin transporter gene （5-HTTLPR） were determined. The 5-HTTLPR （serotonin transporter promoter gene） genotypes in PE patients vs. controls were distributed as follows： L/L 16% vs. 17%, L/S 30% vs. 53% and S/S 54% vs. 28%. We examined the haplotype analysis for three polymorphisms of the 5-HTTLPR gene： LL, LS and SS. The appropriateness of the allele frequencies in the 5-HTTLPR gene was analyzed by the Hardy-Weinberg equilibrium using the Z-test. The short （S） allele of the 5-HTTLPR gene was significantly more frequent in PE patients than in controls （P 〈 0.05）. We suggest that the 5-HTTLPR gene plays a role in the pathophysiology of all primary PE cases. Further studies are needed to evaluate the relationship between 5-HTTLPR gene polymorphism and patient subgroup （such as primary and secondary PE） responses to selective serotonin reuptake inhibitors as well as ethnic differences.

BDNF与5-HTT基因启动子区多态性的交互作用对精神分裂症暴力攻击行为的影响

目的探讨脑源性神经营养因子(BDNF)与5-羟色胺转运体基因启动子区多态性(5-HTTLPR)的交互作用对精神分裂症暴力攻击行为(SCZ-AB)的影响。方法选取169例精神分裂症患者,根据是否有暴力攻击行为分为A组(有暴力攻击行为,n=87)与B组(无暴力攻击行为,n=82)。比较两组一般资料、BDNF与5-HTTLPR基因分型及等位基因频率分布、A组BDNF与5-HTTLPR基因型间Buss&Perry攻击量表和Barratt冲动量表评分,Logistic回归分析不同BDNF基因型和5-HTTLPR基因型对SCZ-AB的影响。运用MDR统计分析不同基因型间交互作用。结果A组与B组间Val和Met频率比较,差异有统计学意义(P<0.05),A组Val/Val频率低于B组(P<0.05),Val/Met和Met/Met基因型频率高于B组(P<0.05);Buss&Perry攻击量表和Barratt冲动量表比较发现:A组Met/Met基因型的各项分值均高于Val/Val、Val/Met基因型(P<0.05);控制性别因素,携带Met等位基因有暴力攻击行为的精神分裂患者的相对危险度是不携带Met等位基因患者的2倍(P<0.05)。Buss&Perry攻击量表和Barratt冲动量表比较发现:L/L基因型患者的各项分值均显著高于S/S基因型(P<0.05)。同时携带Met和L等位基因者的相对危险度是不携带Met和L等位基因者的2倍(P<0.05)。结论同时携带BDNF Met和5-HTTLPR L等位基因患者有暴力攻击行为的危险度较高,BDNF Met等位基因发挥主要作用,Met/Met基因型患者病情更严重。

PcDNA3.1-Tum-5基因真核表达载体的构建

目的构建携带Tum-5基因真核表达载体PcDNA3.1-Tum-5。方法利用巢式PCR扩增人胚肾细胞株HEK293 cDNA获得Tum-5基因,并利用DNA回收试剂盒进行回收;同时扩增、提取pcDNA3.1质粒,并将其与Tum-5基因分别进行EcoRV和XhoI双酶切,回收相应条带,通过T4DNA连接酶进行连接,转化DH5α感受态细胞,获得阳性克隆。获得质粒DNA后行KpnI和XhoI双酶切,克隆并测序酶切产物。结果巢式PCR扩增出的产物与目的基因大小相同;重组质粒经双酶切电泳分析,与预期结果一致;对连接点两端进行测序,结果显示接头两端序列连接正确,插入序列与载体读码框架相匹配。结论本方法可以成功构建人Tum-5基因表达载体,为进一步研究Tum-5基因功能提供了理论依据。

Regulation of demethylation and re-expression of RASSF1A gene in gastric cancer cell lines by combined treatment of 5-Aza-CdR and NaB

AIM： To investigate the changes of methylation state and expression of RASSF1A gene in human gastric cancer cell lines SGC7901 and BGC823 which were treated in vitro with demethlylating agent 5-Aza-CdR in combination with histone deacetylase inhibitor NaB. METHODS： After SGC7901 and BGC823 cells were treated with 5-Aza-CdR and/or NaB, the methylation state of RASSFIA gene was detected by methylationspecific PCR, and the changes in expression of mRNA and protein level of RASSFIA gene were observed by RT-PCR and Western-blotting before and after drug treatment. RESULTS： Hypermethylation was detected in the promoter region of RASSF1A gene in both SGC7901 and BGC823 cells, and there was no expression of this gene at both mRNA and protein level. After treatment with 5-Aza-CdR, demethylation occurred in the promoter region of RASSFIA gene, which subsequently induced re-expression of this gene. The treatment with NaB alone showed no effect on the methylation state and expression of RASSFIA gene. The combined treatment of 5-Aza-CdR and NaB induced complete demethylation of RASSFIA gene, leading to a significantly higher reexpression of the mRNA and protein of RASSFIA than those treated with 5-Aza-CdR alone （P 〈 0.05）. CONCLUSION： Hypermethylation in the promoter region is related to inactivation of RASSFIA gene in human gastric cancer cell lines SGC7901 and BGC823, while demethlylating agent 5-Aza-CdR can reverse the methylation state of RASSF1A gene and induce itsre-expression. Histone deacetylase inhibitor NaB had a synergistic effect with 5-Aza-CdR in both demethylation and gene transcriptional regulation.

Characterizations and identification of the candidate gene of rice thermo-sensitive genic male sterile gene tms5 by mapping

Previous study indicated that the thermo-sensitive genic malesterile(TGMS) gene in rice was regulated by temperature.TGMS rice plays an important role in hybrid rice production,because the application of the TGMS system in two-line breeding is laborsaving,timesaving,simple,inexpensive,efficient,and eliminating the limitations of the cytoplasmic male sterility(CMS) system.'AnnongS' is the first discovered and deeply studied TGMS rice lines in China.'AnnongS-1' and 'Y58S',two derivatives of TGMS line AnnongS,were both controlled by a single recessive gene named tms5,which was genetically mapped on chromosome 2.In this study,three populations('AnnongS-1' × 'Nanjing11','Y58S' × 'Q611',and 'Y58S' × 'Guanghui122') were developed and used for the molecular fine mapping of the tms5 gene.By analyzing recombination events in the sterile individuals using a total of 125 probes covering the tms5 region,the tms5 gene was physically mapped to a 19-kb DNA fragment between two markers 4039-1 and 4039-2,which were located on the BAC clone AP004039.After the construction of the physical map between two markers 4039-1 and 4039-2,a member(ONAC023) of the NAC(NAM-ATAF-CUC-related) gene family was identified as the candidate gene of the tms5 gene.

抗黑素瘤分化相关基因5抗体阳性皮肌炎合并快速进展性间质性肺病的临床特征及危险因素

目的:通过分析抗黑素瘤分化相关基因5抗体(MDA5)阳性皮肌炎(DM)患者合并快速进展性间质性肺病(RPILD)和非RPILD的临床特点差异,探讨合并RPILD发生的危险因素。方法:回顾性分析南京医科大学炎性肌病及结缔组织病相关间质性肺病专病联盟组织收集的251例抗MDA5抗体阳性皮肌炎(MDA5+DM)患者临床资料,将其根据有无合并RPILD进行分组,采用t检验、U检验、χ^(2)检验及Logistic回归分析合并RPILD患者的临床特点,探讨RPILD发生的危险因素。结果:将251例患者分为RPILD组(89例)和非RPILD组(162例),2组患者性别、年龄、病程、红细胞沉降率(ESR)、C反应蛋白(CRP)、抗Ro-52抗体阳性、铁蛋白(SF)、抗MDA5抗体滴度比较,差异均有统计学意义(P<0.05)。单因素Logistic回归分析显示年龄、ESR、抗MDA5抗体滴度、性别(男性)、CRP、抗Ro-52抗体均有统计学意义(OR>1,P<0.05);多因素Logistic回归分析显示性别(男性)、CRP、抗Ro-52抗体有统计学意义(OR>1,P<0.05)。结论:年龄、ESR、抗MDA5抗体滴度可能增加MDA5+DM患者发生RPILD的风险,但不是独立危险因素;性别(男性)、CRP升高、抗Ro-52抗体阳性可能是MDA5+DM患者合并RPILD的独立危险因素,均与RPILD的发生呈正相关。

The 5-HT2c receptor gene Cys23Ser polymorphism influences the intravaginal ejaculation latency time in Dutch Caucasian men with lifelong premature ejaculation

It has been postulated that the persistent short intravaginal ejaculation latency time （IELT） of men with lifelong premature ejaculation （LPE） is related to 5-hydroxytryptamine （HT）2c receptor functioning. The aim of this study was to investigate the relationship of Cys23Ser 5-HT2c receptor gene polymorphism and the duration of IELT in men with LPE. Therefore, a prospective study was conducted in 64 Dutch Caucasian men with LPE. Baseline IELT during coitus was assessed by stopwatch over a 1-month period. All men were genotyped for Cys23Ser 5-HT2c receptor gene polymorphism. Allele frequencies and genotypes of Cys and Ser variants of 5-HT2c receptor gene polymorphism were determined. Association between Cys/Cys and Ser/Ser genotypes and the natural logarithm of the IELT in men with LPE were.investigated. As a result, the geometric mean, median and natural mean IELT were 25.2, 27.0, 33.9s, respectively. Of all men, 20.0%, 10.8%, 23.1% and 41.5% ejaculated within 10, 10-20, 20-30 and 30-60s after vaginal penetration. Of the 64 men, the Cys/Cys and Ser/Ser genotype frequency for the Cys23Ser polymorphism of the 5-HT2c receptor gene was 81% and 19%, respectively. The geometric mean IELT of the wildtypes （Cys/Cys） is significantly lower （22.6s; 95% CI 18.3-27.8s） than in male homozygous mutants （Ser/Ser） （40.4s; 95% CI 20.3-80.4s） （P = 0.03）. It is concluded that Cys23Ser 5-HT2c receptor gene polymorphism is associated with the IELT in men with LPE. Men with Cys/Cys genotype have shorter IELTs than men with Ser/Ser genotypes.