Delivering DNA into Plant Cell by Gene Carriers of ZnS Nanoparticles

The development of nanotechnology provides a new method for genetic engineering.However,the nanoparticles as gene carriers have been mainly used in the mammalian cells so far.We observed that ZnS nanoparticles modified with positively charged poly-L-lysine（PLL） successfully delivered GUS-encoding plasmid DNA into tobacco cells by means of ultrasound-assisted method.Polymerase chain reaction（PCR） detection,Southern blot analysis and GUS histochemical staining were carried out for the regenerated plants.The stable genetic modified plants mediated by ZnS nanoparticles can be obtained.This article demonstrates the great potential of nanoparticles as gene carrier in plant transformation and proves a novel approach for plant genetic decoration.

Genomic Analysis of Mitochondrial Carrier Genes in the Bombyx mori

This study is performed to investigate the mitochondrial carrier gene family in silkworm genome. In total, 30 genes are identified and claded into eight well-conserved groups. Gene duplication contributes to the expansion and complexity of this family. Diverse expression patterns suggest their functional differentiation. Analyses of the sitespecific profiles reveal critical amino acid residues for functional divergence. This study highlights the molecular evolution of the mitochondrial carrier gene family in silkworm and may provide a starting point for further experimental verification.

Enhancement of Immunological Activity of CpG ODN by Chitosan Gene Carrier

To investigate the enhancement of immunological activity of CpG ODN by chitosan gene carrier in mice, the effect of lymphocyte proliferation was detected in mice by using MTT, the levels of IgG and cytokines （IL-2 and IL-12） in serum were measured by ELISA and peripheral blood T lymphocyte subsets CD4^＋, CD8^＋ were analyzed by flow cytometry. Our results showed that spleen lymphocytes isolated from the CS-CpG ODN group of mice showed the strongest proliferation （SI =1.551）, and the levels of IgG, IL-2 and IL-12 in serum were higher than those of other groups. Compared with the immunization with CpG ODN, the immunization with CS-CpG ODN gene carrier was more efficient in up-regulating the percentage of CD4^＋T cells and the ratio of CD4^＋/CD8^＋ of mice, It was concluded that CS gene carrier of CpG ODN was much more effective in improving immunity of CpG ODN in mice.

Structural analysis of DMD gene and its clinical application in Chinese.Ⅰ. Bgl Ⅱ exon-containing fragment,RFLP and carrier detection

This article is one of the serial studies oll the characteristics of the molecular structure for dystrophin gene in Chinese. By using the entire dystrophin cDNA (14 kb) as a probe- the number and RFLPs of Bgl Ⅱ exon-containing fragments of the dystrophin gene were analysed. Four new Bgl Ⅱ fragments were found, two of them (3.7 and 6.2 kb) detected by comparing the hybridization patterns with cDNA1-2a. 1a and 2a, one (9.3 kb) from the hybridization pattern with cDNA 9 by lengthening migrating distance of DNA fragments in electrophoresis. and another one (4.0 kb) by comparing the patterns with cDNA 11-14,11a- 11b’ 11c-12a and 14. The results indicated that the number of Bgl Ⅱ exon-containing fragments should be 59 rather than 55 reported previously, which laid the foundation of the Bgl Ⅱ partial restriction map for dystrophin gene. Three of the four RFLPs found in Caucacian appear in the hybridization patterns of three subclones, i.e.cDNA 2b-3. cDNA 4-5, and cDNA 5b-7.’ The values of expected heterozygote frequency (EHF) were 0.33, 0.33and 0.40 and the observed heterozygote frequency (OHF)were 0.40. 0.40 and 0.48 respectively. Meanwhile, two new rare allelic fragments (15 kb) were found in RFLPs from Bgl Ⅱ/2b-3 and Bgl Ⅱ/4-5a patterns respectively. These Bgl Ⅱ RFLPs and four XbaI RFLPs documented in our laboratory, have been used to detect the carrier in 7 DMDfamilies and 1 BMD family. Of the 69 individuals from the 8 families- 11 females were diagnosed as the carriers with DMD mutation, 4 females as the doubtful carriers, 12 females were defined as normal genotype and 2 females as probably normal. The results suggest that the carrier testing method based on dosage intensity analysis and genotype analysis by using dystrophin cDNA as a probe will be more sensitive and accurate.

小粒径Fe_(3)O_(4)-DMSA-PEI磁性纳米颗粒的制备及其基因负载能力研究

四氧化三铁(Fe_(3)O_(4))磁性纳米颗粒因其制备简单,在外加磁场作用下具有靶向性,并且表面易接枝等特性,可作为被动靶向载体应用于基因治疗领域。本研究采用溶剂热法制备纳米颗粒,并调控堆积生长时间,制得粒径在4~9 nm范围内可控的油相Fe_(3)O_(4)纳米颗粒;使用内消旋-2,3-二巯基丁二酸(DMSA)二次取代其表面的油酸分子,使其具备良好的水相分散性;通过酰胺化反应在其表面接枝支链型聚乙烯亚胺(PEI),最终得到Fe_(3)O_(4)-DMSA-PEI磁性纳米颗粒。研究发现,Fe_(3)O_(4)-DMSA-PEI磁性纳米颗粒的表面Zeta电位高达(52.50±1.94)mV,具有一定的超顺磁性(14.48 emu/g,1 emu/g=1 A·m^(2)/kg)。磁性纳米颗粒与质粒DNA的质量比为15:1时可完全阻滞DNA在凝胶上的电泳,装载量高达6.67%。本研究制备的Fe_(3)O_(4)-DMSA-PEI磁性纳米颗粒具有一定的基因负载能力,有望作为基因载体应用于基因转染领域。

BVDV非结构蛋白NS4B的结构分析及其蛋白表达与鉴定

NS4B是牛病毒性腹泻病毒(Bovine viral diarrhea virus,BVDV)的非结构蛋白,为研究BVDV在病毒侵染宿主细胞过程中的作用,对ns4b进行了结构分析、表达载体构建及蛋白表达。采用Prot-Param、TExpasy和SignalP-4.1等软件分析NS4B蛋白的氨基酸组成、疏水性和空间结构。根据Genebank上公布的BVDVns4b基因序列设计引物,利用PCR方法获得ns4b基因片段,连接到p3×Flag-CMV10表达载体上,构建重组质粒p3×Flag-CMV10-ns4b,经双酶切与测序鉴定正确后,将p3×FlagCMV10-ns4b转染到HEK-293T细胞中,利用Western blot检测NS4B蛋白的表达。结果表明BVDV NS4B蛋白分子量为38.4 kDa,不存在信号肽,有49个磷酸化位点和6个糖基化位点,是一种主要由α-螺旋和无规则卷曲结构组成的疏水性稳定蛋白。成功构建了重组质粒p3×Flag-CMV10-ns4b,并且p3×Flag-CMV10-ns4b在HEK-293T细胞中成功表达,为今后研究NS4B蛋白在BVDV感染宿主细胞及其免疫逃逸机制奠定了基础。

广西来宾市育龄人群珠蛋白生成障碍性贫血基因检测结果分析

目的探讨珠蛋白生成障碍性贫血基因在广西来宾市本地人群的携带率,为来宾市珠蛋白生成障碍性贫血防控工作提供理论依据。方法采用血细胞检测和血红蛋白电泳联合测定对2020年1月~2021年12月在广西来宾市四县一市一区妇幼医院门诊就诊的88152例样本进行珠蛋白生成障碍性贫血筛查,采用多重裂口PCR(gap polymerase chain reaction,Gap-PCR)和反向斑点杂交(reverse dot blot,RBD)等技术,对初筛阳性者进行常见型和罕见型基因检测,并对检测结果进行统计学分析。结果①22553例初筛呈阳性,其中8327例初筛阳性者接受基因诊断,共检出4944例珠蛋白生成障碍性贫血基因携带者,推导出该地区育龄人群总携带率为15.19%,其中α-为3200例(64.73%),β-为1424例(28.80%),αβ复合型为320例(6.47%)。②α-珠蛋白生成障碍性贫血基因携带者中,常见型为3168例(99.00%),罕见型32例(1.00%),共检出13种突变基因和34种基因型,基因型--^(SEA)/αα排在首位。③β-珠蛋白生成障碍性贫血基因携带者中,常见型为1411例(99.09%),罕见型13例(0.91%),共检出19种突变基因和25种基因型,以CD41-42(-CTTT)最为常见。④αβ复合型携带者中共检出53种不同基因型,排在首位的是--^(SEA)/ααβ^(CD41-42M)/β^(N)。⑤瑶族与汉族携带率相当,差异无统计学意义(χ^(2)=0.300,P=0.584),壮族与瑶族、壮族与汉族比较,差异具有统计学意义(χ^(2)=23.66,116.98,均P<0.001)。⑥象州县携带率最高(20.04%),合山市携带率最低(12.38%)。⑦女性携带率(16.56%)高于男性(13.32%),差异有统计学意义(χ^(2)=182.03,P<0.001)。结论来宾地区珠蛋白生成障碍性贫血变异基因类型复杂,该研究首次调查珠蛋白生成障碍性贫血基因在来宾地区人群中的携带率和基因突变谱,为该地区遗传咨询和产前诊断提供了有价值的基线数据。

广州市从化区育龄人群α-珠蛋白生成障碍性贫血筛查及基因鉴定结果分析

目的了解和分析广州市从化区育龄人群中α-珠蛋白生成障碍性贫血发病率及基因突变类型。方法应用血细胞分析和血红蛋白电泳对24083例育龄人群血样进行初筛,初筛阳性者采用跨越断裂点聚合酶链反应(GAP-PCR)和PCR反向点杂交技术检测α-珠蛋白变异基因,使用PCR反向点杂交方法检测β-珠蛋白17种常见突变基因。结果经基因鉴定共检出α-珠蛋白生成障碍性贫血基因异常者2596例,异常发生率10.78%。α-β复合基因突变者170例,复合发生率0.71%。在突变基因中,包括缺失型2550例,占98.23%;非缺失型46例,占1.77%。共含有14种基因突变类型,其中血红蛋白H(HbH)病5种,以--^(SEA)/-α^(3.7)为主;轻型4种,--^(SEA)/αα基因型达到了68.61%;静止型5种,占比最高的前两种基因型为-α^(3.7)/αα和-α^(4.2)/αα。αβ复合基因突变类型检出23种,检出率最高的前六种分别为--^(SEA)/β^(CD41-42),-α^(3.7)/β^(CD41-42),--^(SEA)/β^(654),--^(SEA)/-28,-α^(3.7)/β^(654)和-α^(3.7)/βCD17,占全部复合类型的75.27%。结论广州市从化区α-珠蛋白生成障碍性贫血基因异常发生率较高,基因突变类型和构成比具有自己的特点,是α-珠蛋白生成障碍性贫血一个较为特殊的区域。

脊髓性肌萎缩症携带者筛查及产前诊断结果分析

目的 探索SMA携带者筛查及产前诊断的临床意义。方法 运用实时荧光定量PCR技术进行SMN1基因7号外显子(E7)拷贝数缺失检测,并对结果为阳性的孕妇其配偶进行检测,夫妇均为携带者对胎儿行产前诊断。结果 2472例孕妇共检出SMN1基因E7纯合缺失1例,携带者34例,携带率约为14%。SMA患者女儿诊断为杂合缺失携带者。召回配偶18例,其中1对夫妇检出均为为SMN1基因E7杂合缺失,对其胎儿进行产前诊断未检测到明确致病变异。1例SMA先证者家庭再生育发现:先证者为SMN1基因E7纯合缺失,先证者母亲及父亲为SMN1基因杂合缺失,二胎进行SMA产前诊断,未检测到明确致病变异。结论 本研究通过开展孕妇携带者筛查,可为当地SMA的遗传咨询和产前诊断提供理论依据,并对高风险胎儿使用多技术平台进行产前诊断,可有效避免SMA患儿的出生,对出生缺陷防控具有重要临床指导意义。

Lentivirus vectors construction of SiRNA targeting interference GPC3 gene and its biological effects on liver cancer cell lines Huh-7

Objective:To build GPC3 gene short hairpin interference RNA(shRNA)slow virus veclor.observe expression of Huh-7 GPC3 gene in human liver cell line proliferation apoptosis and the effect of GPC3 gene influencing on liver cancer cell growth,and provide theoretical basis for genc therapy of liver cancer.Methods:Hepatocellular carcinoma cell line Huh-7 wsa transfected by a RNA interference technique.GPC3 gene expression in a variety of liver cancer cell lines was detected by fluorescence quantitative PCR.Targeted GPC3 gene seqnences of small interfering RNA(siRNA)PGC-shRNA-GPC3 were restructured.Stable expression cell linse of siRNA were screened and established with the heplp of liposomes(lipofectamine^(TM2000))as carrier transfcetion of human liver cell lines.In order to validate siRNA interference efficiency.GPC3 siRNA mRNA expression was detected after transfection by using RT-PCR and Western blot.The absorbance value of the cells of blank group,untransfection group and transfection group,the cell cycle and cell apoptosis were calculated,and effects of GPC3 gene nn Huh-7 cell proliferation and apoptosis were observed.Results:In the liver cancer cell lines Huh-7 GPC3 gene showed high expression.PGC-shRNA-GPC3 recombinant plasmid was constructde successfully via sequencing validation.Stable recombinant plasmid transfected into liver cancer cell linse Huh-7can obviously inhibit GPC3 mRNA expression level.Conclusions:The targeted GPC3 siRNA can effectively inhibit the expression of GPC3.

APPLICATION OF GENETIC DEAFNESS GENE CHIP FOR DETECTION OF GENE MUTATION OF DEAFNESS IN PREGNANT WOMEN

Objective The study is to identify the carrier rate of common deafness mutation in Chinese pregnant women via detecting deafness gene mutations with gene chip. Methods The pregnant women in obstetric clinic without hearing impairment and hearing disorders family history were selected. The informed consent was signed. Peripheral blood was taken to extract genom- ic DNA. Application of genetic deafness gene chip for detecting 9 mutational hot spot of the most common 4 Chinese deafness genes, namely GJB2 （35delG, 176del16bp, 235delC, 299delAT）, GJB3 （C538T） ,SLC26A4 （ IVS72A〉G, A2168G） and mito- chondrial DNA 12S rRNA （A1555G, C1494T） . Further genetic testing were provided to the spouses and newborns of the screened carriers. Results Peripheral blood of 430 pregnant women were detected, detection of deafness gene mutation carri- ers in 24 cases（4.2%）, including 13 cases of the GJB2 heterozygous mutation, 3 cases of SLC26A4 heterozygous mutation, 1 cases of GJB3 heterozygous mutation, and 1 case of mitochondrial 12S rRNA mutation. 18 spouses and 17 newborns took further genetic tests, and 6 newborns inherited the mutation from their mother. Conclusion The common deafness genes muta- tion has a high carrier rate in pregnant women group, 235delC and IVS7-2A〉G heterozygous mutations are common.

Cloning and characterization of a stearoyl-ACP desaturase gene from Jatropha curcas

Using degenerate primers and RT-PCR, RACE techniques, a 1491 bp cDNA segment of stearoyl-acyl carrier protein desaturase （SAD） is cloned from developing seeds of Jatropha curcas L. The segment contains a 1191 bp of complete open reading frame （ORF）. Analysis in the BLAST on NCBI shows that Jatropha curcas SAD （JSAD） gene encodes a protein precursor composed of a signal peptide of 33 amino acids and a mature peptide of 363 amino acids. The homological analysis shows that JSAD has high level of homology both in nucleotide sequence and in amino acid sequence to other plants SADs. The nucleotide and peptide identity of JSAD to Ricinus communis SAD （RSAD） is up to 89% and 96.2% respectively. Molecular modeling of JSAD indicates that its three-dimensional structure strongly resembled the crystal structure of RSAD.

Applying a highly specific and reproducible cDNA RDA method to clone garlic up-regulated genes in human gastric cancer cells

AIM: To develop and optimize cDNA representationaldifference analysis (cDNA RDA) method and to identify andclone garlic up-regulated genes in human gastric cancer(HGC) cells.METHODS: We performed cDNA RDA method by usingabundant double-stranded cDNA messages provided by twoself-constructed cDNA libraries (Allitridi-trested and paternalHGC cell line BGC823 cells cDNA libraries respectively).BamH Ⅰ and Xho I restriction sites harbored in the libraryvector were used to select representations. Northern andSlot blots analyses were employed to identify the obtaineddifference products.RESJLTS: Fragments released from the cDNA library vectorafter restriction endonuclease digestion acted as goodmarker indicating the appropriate digestion degree for libraryDNA. Two novel expressed sequence tags (ESTs) and arecombinant gene were obtained. Slot blots result showed a8-fold increase of gila-derived nexin/protease nexin 1 (GDN/PN1 ) gene expression level and 4-fold increase of hepatitis Bvirus x-interacting protein (XIP) mRNA level in BGC823 cellsafter Allitridi treatment for 72 h.CONCLUSION: Elevated levels of GDN/PN1 and XIP mRNAsinduced by Allitridi provide valuable molecular evidence forelucidating the garlic' s efficacies against neurodegenerativeand inflammatory diseases. Isolation of a recombinant geneand two novel ESTs further show cDNA RDA based on cDNAlibraries to be a powerful method with high specificity andreproducibility in cloning differentially expressed genes.

Human umbilical cord mesenchymal stem cells as cell carriers in the treatment of gliomas: research status and prospects

Human umbilical cord mesenchymal stem cells(HuMSCs)have the multi-difFerentiation potential to differentiate into various types of cells without immune rejection.They are considered to be an ideal source of neural stem cells and also an ideal cell carrier for gene therapy.Because of the invasive growth of brain gliomas,most of them have no obvious boundaries with normal brain tissues.It is difficult to completely remove them by surgery and the remaining cells become the main source of tumor recurrence.In recent years,gene therapy has become a new method for the treatment of gliomas.The vector carrying the target gene is introduced into HuMSCs in a certain way to correct gene defects or play other roles.The differentiation potential of HuMSCs makes it an ideal source of nerve cells to play a greater role in gene therapy of glioma.Therefore,this article reviews the current status and prospects of HuMSCs as cell carriers in the treatment of glioma.

不同来源肠炎沙门菌耐药特征及遗传多样性特点的研究

目的分析福建地区腹泻病人和表观健康人群携带的肠炎沙门菌耐药特征及遗传多样性特点。方法收集福建地区腹泻患者和表观健康人群携带的肠炎沙门菌,采用K-B法进行药敏实验,PCR扩增毒力基因,多位点融数目亭联重复序列分析(multiple-locus variable-number tandem repeat analysis,MLVA)技术进行分子分型,并应用BioNumerics软件进行聚类分析。结果福建地区肠炎沙门菌除对CIP和NOR 100%敏感外,对其他8种药物(AMP、AMC-AC、CTX、CRO、CHL、NAL、SXT和TET)均有不同程度的耐药。腹泻患者分离株的多重耐药率(33.33%)高于表观健康人群分离株(15.22%)。10种毒力基因(sitC、hilA、sseL、sifA、mgtC、siiE、sopB、stn、spvB和pefA)均有检出,且其在腹泻患者和表观健康人群分离株中分布不同。毒力基因谱型54个(VP1~VP54),其中VP3只存在于表观健康人群分离株,且为其优势谱型,占比为13.04%;VP4和VP5只存在于腹泻患者分离株;VP4和VP3、VP1均为腹泻患者分离株中的优势谱型,占比均为11.90%。所有分离株共分为40个MLVA型(MT0001~MT0040)、2个主要基因簇(clusterⅠ和clusterⅡ),其中clusterⅡ包含的菌株均来自表观健康人群;clusterⅠ包含的菌株来自及腹泻患者和表观健康人群。结论福建地区肠炎沙门菌呈现遗传多态性,腹泻患者分离株的耐药性和致病力均高于表观健康人群分离株。

siRNA非病毒载体递送用于肿瘤治疗的研究进展

近年来基于RNA干扰(RNA interference,RNAi)的基因治疗技术在肿瘤治疗方面引起广泛关注。在常规药物治疗无效的情况下,RNAi为癌症患者带来了新的希望。但是,由于小分子干扰RNA(small interfering RNA,siRNA)在体内存在易降解、难递送等问题,极大地限制了其临床转化潜力。纳米载体以其独特的尺寸效应和多样的修饰策略,能够介导高效、靶向的RNA递送,以实现其基因沉默。本文综述了RNAi在基因治疗中的作用机制以及体内递送siRNA的不同载体,介绍了载体体内递送siRNA的主要障碍和作用靶点,并比较了不同载体在siRNA递送中的优势和不足,为新载体的设计提供借鉴,推动RNA干扰疗法向临床的转化。

澳洲坚果光壳种MiSAD的克隆与表达

澳洲坚果果仁中含有丰富的不饱和脂肪酸(unsaturated fatty acid,UFA),其不饱和脂肪酸生物合成的分子机制还有待进一步解析。植物硬脂酰-酰基载体蛋白脱饱和酶(SAD)是脂肪酸生物合成途径中形成不饱和脂肪酸的关键酶。本研究以澳洲坚果(Macadamia integrifolia)光壳种为对象,通过PCR技术克隆获得澳洲坚果硬脂酰-酰基载体蛋白脱饱和酶基因(MiSAD),并对结构功能和表达模式进行了初步分析。结果显示,克隆获得5923 bp的MiSAD基因组DNA序列,该基因由3个外显子2个内含子组成,包含1191 bp的编码框,与公布的粗壳种MtSAD序列高度一致;编码396个氨基酸;MiSAD分子量为45.22 kDa,等电点为5.93,属于酰基-ACP脱饱和酶,是位于叶绿体或质体基质中的水溶性酶;高度保守的区域存在形成酶活位点的2个E-X-X-H二铁原子中心基序,N端和C端氨基酸序列差异较大;二级结构中以α-螺旋和无规则卷曲为主;三级结构预测中存在形成脂酰链结合部位的螺旋-转角-螺旋(HTH);与蒂罗花的同源性最高达94.2%,与其他物种的SAD同源性也都在80%以上;分子进化树显示与荷花进化关系较近,属于植物脂酰-ACP脱饱和酶。荧光定量PCR数据显示MiSAD在根、茎、叶、花、果中均有表达,其中叶片和果实中表达量较高,果实中的MiSAD表达量在开花后第100天左右达到最高,之后随着果实的成熟逐渐下降,呈现正态分布趋势。该研究为深入研究MiSAD在澳洲坚果果仁中不饱和脂肪酸生物合成的作用机制奠定基础。

小鼠TDO2基因条件性敲除打靶载体的构建

目的构建小鼠TDO2基因条件性敲除打靶载体,为建立TDO2基因条件性敲除小鼠奠定基础。方法根据CRISPR/Cas9技术原理,设计并构建单链向导RNA(sgRNA)和Donor载体,以TDO2-201(ENSMUST00000029645.13)转录本的外显子3作为敲除区,在打靶基因两侧各放置一个Loxp元件,建立条件性敲除TDO2第3号外显子的条件性基因打靶载体。将CRISPR/Cas9复合体和Donor载体显微注射到C57BL/6小鼠的受精卵中,获得阳性F0小鼠,再将阳性F0代小鼠与C57BL/6小鼠交配获得F1代小鼠,并经PCR和基因测序鉴定F1代小鼠基因型。结果结果证实所构建的TDO2基因条件性敲除打靶载体符合设计要求,成功繁育并鉴定出B6/JGpt-TDO2^(em1C)flox/Gpt小鼠。结论成功构建了小鼠TDO2基因条件性敲除打靶载体,为后续进一步构建TDO2基因条件敲除小鼠奠定了基础。

温州地区3620例孕妇耳聋基因产前筛查及临床意义分析

目的 分析温州地区3 620例孕妇常见遗传性耳聋基因突变筛查情况,探讨温州地区听力正常孕妇进行耳聋基因携带者筛查的临床意义。方法 选取2020年2月1日至2022年7月31日在温州市中心医院就诊的3 620例听力正常、无耳聋家族史的孕妇为研究对象,采用PCR+导流杂交法检测GJB2、GJB3、SLC26A4以及线粒体12S rRNA 4个遗传相关耳聋基因的21个位点。当夫妻双方为相同耳聋基因突变携带者时,予遗传咨询及生育指导。结果 3 620例孕妇中共检出耳聋基因携带者163例(4.50%);检出5种GJB2基因突变共85例,其中c.235delC 65例;检出6种SLC26A4基因突变共44例,其中IVS7-2A>G 33例;检出线粒体12S rRNA携带者15例,GJB3携带者19例。对孕妇为GJB2或SLC26A4携带者的配偶进行召回行相应基因Sanger测序,结果 8例为携带者,其中7例接受产前诊断,其中胎儿1例c.235delC纯合突变,1例SLC26A4 IVS7-2A>G合并c.2168A>G复合杂合突变,患者选择终止妊娠。结论 温州地区听力正常孕妇常见耳聋基因携带率为4.50%,且以GJB2 c.235delC、SLC26A4 IVS7-2A>G位点为主,对温州地区孕妇行常见耳聋基因筛查、遗传咨询及产前诊断是耳聋精准防控的有效方法。

牦牛MPC1和MPC2基因克隆及其组织表达特征分析

【目的】明确牦牛线粒体丙酮酸载体编码基因(MPC1和MPC2)的分子生物学特性及其组织表达特征,为揭示MPC基因在牦牛适应高原环境和能量代谢中的作用机制提供理论依据。【方法】选取麦洼牦牛为研究对象,PCR扩增牦牛MPC1和MPC2基因编码区(CDS)序列,利用在线生物信息学分析软件预测其蛋白结构及理化性质,并以实时荧光定量PCR检测MPC1和MPC2基因在不同年龄(0.5、1.5和2.5岁)牦牛各组织中的表达情况。【结果】牦牛MPC1基因CDS序列长330 bp,共编码109个氨基酸残基;MPC2基因CDS序列长384 bp,共编码127个氨基酸残基。基于MPC1和MPC2基因CDS序列相似性构建的系统发育进化树显示,牦牛分别与黄牛和水牛的亲缘关系最近,与绵羊的亲缘关系最远。牦牛MPC1和MPC2蛋白均为稳定的亲水性蛋白,丙氨酸和亮氨酸含量较高,有跨膜结构但无信号肽,均存在1个MPC结构域;其二级结构以α-螺旋为主(分别占57.80%和55.12%),三级结构模型为5xpd.1.A。MPC1和MPC2基因在2.5、1.5和0.5岁牦牛心脏中的相对表达量均最高,其次是肾脏和肝脏,而在脾脏中的相对表达量最低;MPC1和MPC2基因在不同年龄段牦牛各组织中的表达趋势不一致,可能与基因表达的组织特异性及二者在牦牛不同生长发育阶段发挥的作用不同有关。【结论】MPC1和MPC2基因在反刍动物间具有高度的保守性,其表达存在组织特异性和时序性,尤其在心脏中高表达,且编码蛋白中富含丙氨酸和亮氨酸,说明MPC1和MPC2基因在牦牛改善肉品质及适应高原环境的过程中扮演着重要角色,但二者在牦牛不同生长发育阶段发挥的作用有所差异。