RDH12-associated retinal degeneration caused by a homozygous pathogenic variant of 146C>T and literature review

AIM:To describe the clinical,electrophysiological,and genetic features of an unusual case with an RDH12 homozygous pathogenic variant and reviewed the characteristics of the patients reported with the same variant.METHODS:The patient underwent a complete ophthalmologic examination including best-corrected visual acuity,anterior segment and dilated fundus,visual field,spectral-domain optical coherence tomography(OCT)and electroretinogram(ERG).The retinal disease panel genes were sequenced through chip capture high-throughput sequencing and Sanger sequencing was used to confirm the result.Then we reviewed the characteristics of the patients reported with the same variant.RESULTS:A 30-year male presented with severe early retinal degeneration who complained night blindness,decreased visual acuity,vitreous floaters and amaurosis fugax.The best corrected vision was 0.04 OD and 0.12 OS,respectively.The fundus photo and OCT showed bilateral macular atrophy but larger areas of macular atrophy in the left eye.Autofluorescence shows bilateral symmetrical hypo-autofluorescence.ERG revealed that the amplitudes of a-and b-wave were severely decreased.Multifocal ERG showed decreased amplitudes in the local macular area.A homozygous missense variant c.146C>T(chr14:68191267)was found.The clinical characteristics of a total of 13 patients reported with the same pathologic variant varied.CONCLUSION:An unusual patient with a homozygous pathogenic variant in the c.146C>T of RDH12 which causes late-onset and asymmetric retinal degeneration are reported.The clinical manifestations of the patient with multimodal retinal imaging and functional examinations have enriched our understanding of this disease.

外源添加VB_(12)对肺炎克雷伯氏菌代谢3-羟基丙酸的影响

为了探究外源添加维生素B12(Vitamin B12,VB_(12))对Klebsiella pneumoniae HD79和K.pneumoniae HD79-T利用甘油还原途径生产3-羟基丙酸(3-hydroxypropionic acid,3-HP)的影响以及摸索VB_(12)对K.pneumoniae HD79和K.pneumoniae HD79-T的阈值上限,将不同浓度(0.01、0.02、0.03、0.04、0.05 g/L)的VB_(12)添加到K.pneumoniae HD79及K.pneumoniae HD79-T的发酵培养基中,利用HPLC检测其底物消耗及产物产生情况、qRT-PCR检测还原途径相关基因的mRNA表达情况以及酶联免疫试剂盒检测代谢相关酶活性。结果表明,VB_(12)对K.pneumoniae HD79和K.pneumoniae HD79-T的阈值为0.01 g/L和0.03 g/L。与未添加VB_(12)相比,菌株K.pneumoniae HD79和K.pneumoniae HD79-T的3-HP产量分别提高了24.39%,8.86%;醛脱氢酶基因puuC表达量分别提高了2.49倍和1.68倍;ALDH、GDHt和PDOR的酶活力分别提高了50.24%、40.36%和18.29%,及30.49%、37.84%和13.56%。说明通过外源添加辅酶因子VB_(12)对肺炎克雷伯氏菌高产3-HP是可行策略。

Identification of sika deer and red deer using partial cytochrome b and 12s ribosomal RNA genes

A study was conducted on the identifications of the degraded samples of sika deer （Cervus nippon） and red deer （Cervus elaphus） by phylogenetic and nucleotide distance analysis of partial Cytb and 12s rRNA genes sequences. 402 bp Cytb genes were achieved by PCR-sequencing using DNA extracted from 8 case samples, and contrasted with 27 sequences of Cytb gene downloaded from GenBank database. The values of three nucleotide distance between three suspected samples and sika deer were identical （0.026±0.006）, which was smaller than the smallest nucleotide distance between eastern red deer and sika deer （0.036）. Furthermore, phylogenetic analysis of sika deer and red deer indicated that the evidences located within the same cluster as sika deer. The evidences were sika deer materials. As the same way, other three suspected samples were derived from red deer. The results were further confirmed by phylogenetic and nucleotide distance analysis of 387 bp 12s rRNA gene. The method was powerful and less time-consuming and helpful to reduce the related cases with wildlife.

Phylogenetic Relationships among 12 Species of Tetrigidae (Orthoptera:Tetrigoidea) Based on Partial Sequences of 12S and 16S Ribosomal RNA

Mitochondrial 12S and 16S ribosomal RNA genes sequences were sequenced using dye-labeled terminator on an ABI 377 automated sequencer in 11 individuals and 1 species' sequences were gained from GenBank,representing 6 genera of family Tetrigidae.The collated sequences were aligned using Clustal X version 1.81 and then,the sequence variability and heredity distances based on Kimura 2-parameter model were calculated using Mega 2.1.In obtained sequences (736 bp),the average A+T content is 73.9%,ranging from 71.2% to 77.5%;the overall G+C content is 26.1%,ranging from 22.5% to 28.8%.Based on alignment of the combined sequences,185 parsimony-informative sites were revealed in 755 available base pairs.Phylogenetic trees were reconstructed using NJ,MP and ML methods with Cylindraustralia kochii as outgroup.The results indicated that the monophyletic nature of Tetrix is questioned and suggest that T.tubercarina may be given tribal rank.Our results also show that Coptltettix huanjiangensis and C.gongshanensis are the same species,i.e.Coptltettix gongshanensis Zheng,and C.huanjiangensis is the synonyms of C.gongshanensis.

Cloning of Cotton Delta-12 Oleate Desaturase Gene FAD2-1 and Construction of Its ihpRNA and amiRNA Interference Vectors

Delta-12 oleate desaturase gene （FAD2-1） which converts oleic acid into linoleic acid, is the key enzyme determining the fatty acid composition of cottonseed oil. By employing RT-PCR method, full length cDNA of cotton delta-12 oleate desat- urase gene GhFAD2-1 containing an open reading frame of 1 158 bp was cloned for constructing RNAi vector. A 515 bp long specific fragment of this gene was se- lected for constructing ihpRNA vector under the control of a seed-specific promoter NAPIN, named pFGC1008-NAPIN-FAD2-1; meanwhile miRNA gene-silencing vector pCAMBIA1302-amiRNA-FAD2-1 targeting GhFAD2-1 was also constructed.

猪产业链中鼠伤寒沙门菌及沙门菌血清型4,[5],12:i:-基因组学分析

旨在探究鼠伤寒沙门菌及沙门菌血清型4,[5],12:i:-基因组学特征。采用Illumina NovaSeq 6000平台对91株河南省猪产业链中鼠伤寒沙门菌及沙门菌血清型4,[5],12:i:-分离菌进行全基因组测序,通过生物信息学分析,进行其血清型的预测、多位点序列的分型以及质粒类型、耐药基因和毒力基因分析。结果表明,在河南省猪产业链中沙门菌4,[5],12:i:-的流行率(1.58%,50/3173)已经超过鼠伤寒沙门菌的流行率(1.29%,41/3173);91株沙门菌的序列型分为ST34(71.42%,65/91)和ST19(28.57%,26/91);鼠伤寒沙门菌/ST34菌株和4,[5],12:i:-/ST34菌株都是IncHI2A_1、IncHI2_1和Col440I_1质粒的偏好宿主;沙门菌血清型4,[5],12:i:-携带率较高的耐药基因是blaTEM-1B_1(72%)、tet(B)_2(90%)、sul2_3(66%)、blaOXA-1_1(34%)等;相比鼠伤寒沙门菌菌株,沙门菌血清型4,[5],12:i:-菌株中质粒的携带率更高,且携带更多种类的耐药基因和毒力基因。本研究首次证实,河南省猪产业链中沙门菌血清型4,[5],12:i:-的流行已经超过鼠伤寒沙门菌,在一定程度上解释了该血清型在河南省病人中主要流行的原因。

广西地区壮族正常听力人群线粒体基因12S rRNA的突变研究

目的研究广西地区壮族正常听力人群线粒体基因12S rRNA的突变携带率以及突变特点,为临床防聋及治聋提供参考。方法采用晶芯十五项遗传性耳聋基因检测试剂盒(微阵列芯片法)对广西地区150例壮族正常听力的受试者进行线粒体基因12S rRNA的2个突变位点检测,对确诊的阳性结果进行Sanger测序分析。结果150例受试者中,检出线粒体基因12S rRNA 1555 A>G突变者1例(携带率为0.67%),经Sanger测序证实为1555 A>G突变,未发现1494C>T位点突变。结论在广西地区壮族人群中开展线粒体基因12S rRNA突变筛查具有重要意义,可以为突变携带者及其母系亲属提供合理的用药指导、遗传咨询,是预防药物性聋的有效措施。

Construction of retroviral vector of p^(125FAK) specific ribozyme genes and its effects on BGC-823 cells

AIM： To construct the retroviral vector of p^125FAK specific ribozyme genes and to explore the feasibility of ribozyme in BGC-823 gene therapy in vitro. METHODS： A hammerhead ribozyme DNA targeting p^125FAK mRNA from nt 1010 to nt 1032 was synthesized and recombinated into the retroviral vector pLXSN forming pLRZXSN recon. Using the lipofectin-mediated DNA transfection technique, pLRZXSN was introduced into BGC-823 cells. The effects of ribozyme on the growth of BGC-823 cells and apoptosis were studied by cell colony assay, flow cytometry （FCM）, reverse transcriptasepolymerase chain reaction （RT-PCR）, detection of DNA fragmentation and electron microscopy. RESULTS： The number of BGC-823 cell colonies was inhibited by 56% after the cells were treated for 48 h. The cell proliferation was inhibited effectively by p^125FAK ribozyme and the inhibitory effect depended on the concentration and the time of incubation. The expression of p^125FAK mRNA and protein p^125 decreased sharply in BGC-823 cells treated with p^125FAK ribozyme. The characteristics of apoptosis, namely sub-G1 peak, DNA fragmentation and morphological changes, were revealed in BGC-823 cells treated with p^125FAK ribozyme. CONCLUSION： p^125FAK ribozyme decreases p^125FAK gene expression and induces apoptosis of human gastric cancer cells in vitro.

THE INFLUENCE OF HUMAN SINGLE CHAIN INTELEUKIN-12 GENE TRANSDUCTION ON THE BIOLOGICAL BEHAVIOR OF HEPATOMA 7721 CELLS

Objective. To investigate the anti- tumor effects of human single chain interleukin- 12 (hscIL- 12). Method. pcDNA/ hscIL- 12 recombinant was transfected into human hepatic carcinoma cells (7721 cells) by lipofectin method. The 7721/hscIL- 12 cells which secrete hscIL- 12 stably, were obtained via G418 selection, and in vitro the influence of hscIL- 12 gene transduction on the growth of tumor cells was evaluated by cell cycle analysis. In vivo, genetically engineered 7721 cells (7721/hscIL- 12, 7721/pcDNA) and parental cells were implanted into BALB/c nude mice,respectively. 7721/pcDNA and 7721/hscIL- 12 groups were divided into two sub- groups on day 8: one was administered with hPBL twice, 6 days at interval; the other was given equal volume of PBS. Mice were sacrificed on day 26, and spleens and tumors were taken out for histologic assay. Results. hscIL- 12 produced stably by 7721/hscIL- 12 cells had bioactivity, and it was proved by Western blot, immunocytochemistry, and in situ hybridization. In vitro, compared with 7721 and 7721/pcDNA, the 7721/hscIL- 12 grew much more slowly. FACS assay showed apparent G1 arrest of 7721/hscIL- 12 cells. In animal experiment, on day 8 after inoculation, the tumors of 7721 and 7721/pcDNA group were up to 5～ 7mm,while those of 7721/hscIL- 12 group were 2～ 4mm.When treated with hPBL, the tumor of 7721/hscIL- 12 group disappeared completely. Histologically, the tumors from 7721/hscIL- 12 without hPBL treatment had numerous lymphocyte infiltration, the tumor cells displayed depression looking, atrophy, focal necrosis and apoptosis , whereas the tumors of 7721 and 7721/pcDNA groups grew thrivingly. Conclusion. hscIL- 12 transduced 7721 cells could induced significant antitumor immune response which resulted in tumor regression totally when the hPBL was inoculated, and also hscIL- 12 has certain effects on mice immune system. These findings suggest that hscIL- 12 and hscIL- 12 gene therapy might have promising prospects in clinical application.

Frequency of mitochondrial 12S rRNA gene A1555G and 961 insC mutations among children with sensorineural deafness in China

Objective： To investigate the frequency of mitochondrial 12S rRNA gene A1555G and 961 insC mutations among Chinese with sensorineural deafness. Methods： Blood samples from 78 sporadic cases with sensorineural deafness were obtained and DNA was extracted from the leukocytes, then the mitochondrial DNA target fragments were amplified by polymerase chain reaction（PCR）. The 1555G mutations were detected by BsmA 1 restriction endonuclease digestion, every fragment was analyzed by sequencing; All the 961 insC mutation were detected by direct sequencing. Results： The percent age of A1555G mutation and mt961C insertion were 6.4% and 2.6% in the hearing-impaired Chinese subjects respectively. Conclusion： A1555G and 961insC mutations in mitochondrial DNA 12S rRNA gene regions may play a role in the pathogenesis of hearing loss in the sporadic cases.

Protective effects of proanthocyanidins on beta-amyloid peptide (25-35)-induced PC12 cell apoptosis by blocking S-phase and increasing p53 gene expression

BACKGROUND： Current studies related to the effects of proanthocyanidins on Alzheimer＇s disease have focused primarily on the signal transduction pathway of cellular apoptosis. However, the influence of p53 gene expression on cell cycle regulation, with regard to the protective mechanisms of proanthocyanidins, has not been reported. OBJECTIVE： To observe the effect of proanthocyanidins on cell cycle distribution, cellular apoptosis and p53 gene expression in β-amyloid peptide （25-35） （Aβ25-35）-induced PC12 cells cultured in serum-free media, and to investigate the molecular neuroprotective mechanisms of proanthocyanidins with regard to cell cycle regulation. DESIGN, TIME AND SETTING： A parallel, controlled, at the Institute of Biochemistry and Molecular Biology cellular, and molecular study was performed Guangdong Medical College from July 2006 to July 2008. MATERIALS： Proanthocyanidins were provided by Nanjing Xuezi Medical and Chemical Research Center, China; Aβ25-35 was provided by Sigma, USA; PC12 cells were provided by the Institute of Basic Medical Science, Academy of Military Medical Sciences; and rabbit anti-p53 polyclonal antibody was provided by Santa Cruz Biotechnology, USA. METHODS： PC12 cells were cultured in serum-free media for 24 hours. Cells from the model group were treated with 25 μmol/L Aβ25-35 for 24 hours. Cells in the drug protection group were pre-treated with 30 mg/L proanthocyanidins for 1 hour and then treated with 25 μmol/LAβ2^-35 for 24 hours. The control group was not treated. MAIN OUTCOME MEASURES： Flow cytometry was used to detect cell cycle distribution and rate of apoptosis; reverse-transcriptase polymerase chain reaction was used to detect p53 mRNA expression; and Western blot was used to detect p53 protein expression. RESULTS： After treating with 25 μmol/LAβ25-35 for 24 hours, the rate of apoptosis and the percentage of cells in S phase were significantly increased （P 〈 0.01 ）, and p53 mRNA and protein expressions were decreased. Pretreatment with proanthocyanidins for 1 hour blocked the increase in apoptosis and the percentage of cells in S phase in Aβ25-35-induced PC12 cells （P 〈 0.01 ） and increased p53 mRNA and protein expressions. CONCLUSION： Proanthocyanidins blocked apoptosis and S-phase arrest in Aβ25-35-induced PC12 cells cultured in serum-free media. The protective mechanism could be related to increased p53 mRNA and protein expressions.

Effect of the Antisense BcMF12 Driven by the BcA9 Promoter on Gene Silencing in Brassica campestris L.ssp.chinensis

The study analyzed the silencing of BcMF12 gene regulated by BcA9 promoter in the transgenic pakchoi and confirmed the effect of antisense BcMF12 gene on the pollen development. A conserved BcMF12 gene fragment was amplified from the cDNA of flower buds in pakchoi （Brassica campestris L. ssp. chinensis, syn. B. rapa L. ssp. chinensis） and was fused to the anther specific BcA9 promoter. The plant antisense expression vector was constructed and then introduced into pakchoi via Agrobacterium-mediated transformation. The transgenic plants were screened by antibiotics and molecular analysis. PCR and Southern blot revealed that the antisense BcMF12-GUS fusion gene regulated by BcA9 promoter was integrated into transgenic plants. Northern blot suggested that the expression of BcMF12 gene was down-regulated significantly. The pollen germination rate of transgenic plants with antisense BcMF12 gene decreased as compared with that of the control plants. The expression of the gene BcMF12 related to the pollen development was inhibited by the antisense BcMF12 driven by BcA9 promoter, which consequently affected the pollen development in pakchoi.

1株产VB_(12)球形赖氨酸芽孢杆菌C5.1的分离、全基因组测序及分析

为深入探究球形赖氨酸芽孢杆菌C5.1(Lysinibacillus sphaericus C5.1)菌株产VB_(12)的作用机制,利用PacBio Sequel和Illumina NovaSeq PE150相结合的方法对C5.1菌株进行全基因组测序,并对测序数据进行拼接、基因预测及功能注释。结果表明,C5.1菌株基因组为一个环状DNA,不含质粒,大小为4690817 bp,GC含量为37.21%,预测得到4756个编码基因,111个tRNA基因和34个rRNA基因。通过基因本体论、直系同源集、京都基因与基因组百科全书和转运蛋白分类数据库对C5.1菌株基因组进行注释分析,分别匹配到3095、3182、4374个和397个基因。进一步分析发现C5.1菌株基因组中包含从尿卟啉原Ⅲ逐步转化合成VB_(12)的关键酶。本研究为解析C5.1菌株在臭腐乳发酵过程中的代谢机理提供遗传信息基础,也为今后开展发酵食品中VB_(12)的生物合成机制研究提供理论支撑。

Combination therapy of murine liver cancer with IL-12 gene and HSV-TK gene

Objective: To investigate the synergistic anti-tumor effects of murine IL-12 gene and HSV-TK gene therapy in mice bearing liver cancer. Methods: Mouse liver cancer MM45T. Li (H-2d) cells were transfected with retroviral vector containing IL-12 gene or HSV-TK gene insert. Gene-modified liver cancer cells, MM45T. Li/IL-12 and MM45T. Li/TK, with stable expression of IL-12 and TK were obtained. Balb/c mice were inoculated subcutaneously with 2′105 MM45T. Li cells. When the tumor reached a size of 0.5-1.0 cm, a mixture of MM45T.Li/TK cells and 60Co-irradiated MM45T. Li/IL-12 cell were injected intratumoraly. Ganciclovir (GCV) was injected ip (40 mg.kg-1.d-1) for 10 days. Intratumoral injection of 60Co-irradiated MM45T. Li/IL-12 cells was repeated twice in one week apart. Mice with distant tumors were treated according to the same protocol. CTL activity of spleen cells was measured by 51Cr-release assay and phenotype of tumor infiltrating lymphocytes by immunohistochemical staining. Results: In mice treated with MM45T. Li/IL-12 or MM45T. Li/TK+GCV individually led to moderate reduction in tumor growth, but neither could eradicate the tumor completely, while in 60% of mice treated with a mixture of MM45T. Li/IL-12 and MM45T. Li/TK cells plus GCV, complete tumor regression was observed, with no tumor recurrence for two months. The growth of distant tumor was also inhibited significantly in mice similarly treated. Most of the mice received combined gene therapy plus GCV had abundant CD4+, CD8+T lymphocyte infiltration. Their CTL activity was significantly higher than in mice received single gene therapy. Conclusion Combination therapy with IL-12 gene and HSV-TK gene plus GCV is effective for mouse liver cancer.

A phylogeny of the Passerida(Aves: Passeriformes)based on mitochondrial 12S ribosomal RNA gene

Background: Passerida is the largest avian radiation within the order Passeriformes. Current understanding of the high-level relationships within Passerida is based on DNA–DNA hybridizations; however, the phylogenetic relationships within this assemblage have been the subject of many debates.Methods: We analyzed the 12 S ribosomal RNA gene from 49 species of Passerida, representing 14 currently recognized families, to outline the phylogenetic relationships within this group.Results: Our results identified the monophyly of the three superfamilies in Passerida: Sylvioidea, Muscicapoidea and Passeroidea. However, current delimitation of some species is at variance with our phylogeny estimate. First, the Parus major, which had been placed as a distinct clade sister to Sylvioidea was identified as a member of the super family;second, the genus Regulus was united with the Sturnidae and nested in the Muscicapoidea clade instead of being a clade of Passerida.Conclusion: Our results were consistent with Johansson's study of the three superfamilies except for the al ocation of two families, Paridae and Regulidae.

Development of Molecular Marker Linked to Cf-10 Gene Using SSR and AFLP Method in Tomato

The leaf mould resistance gene Cf-10 on tomato confered resistant or immune to all prevalent physiological races of Cladosporium fulvum presented in three northeastern provinces of China in inoculation test. In order to better utilize Cf-10 gene in a marker-assisted selection program and to permit the pyramiding of one or several resistance genes in a cultivar, tightly linked SSR and AFLP markers were obtained by the bulked segregant analysis method. One SSR marker and three AFLP markers were identified linked to Cf-10 gene, with the distance of 9.73, 5.8, 8.5, and 10.6 cM, respectively. These markers will facilitate the selection of resistant tomato germplasm containing Cf-10 gene.

LncRNA SNHG12在宫颈癌中的表达及其与高危型HPV感染的相关性研究

目的探讨长链非编码RNA小核仁RNA宿主基因12(LncRNA SNHG12)在宫颈癌组织中的表达情况,分析其与高危型人乳头瘤病毒(HR-HPV)感染的相关性。方法前瞻性选取2018年2月至2020年3月张家口市第一医院收治的宫颈癌患者120例为宫颈癌组,另纳入同期宫颈上皮内瘤变(CIN)患者120例为CIN组及同期本院健康体检女性志愿者120名为对照组。其中CINⅠ49例,CINⅡ30例,CINⅢ41例;FIGOⅠ、Ⅱ期87例,FIGOⅢ期33例。实时荧光定量聚合酶链反应法检测LncRNA SNHG12在3组宫颈组织中的表达水平;Spearman相关性分析LncRNA SNHG12表达与HR-HPV感染的相关性;多因素Logistic回归分析影响宫颈癌发生病变的因素。结果FIGOⅢ期组(90.91%)、FIGOⅠ、Ⅱ期组(86.21%)HR-HPV感染率高于CINⅢ组、CINⅡ组、CINⅠ期组及对照组,CINⅢ期组(73.17%)、CINⅡ期组(63.33%)HR-HPV感染率高于CINⅠ组和对照组,CINⅠ期组HR-HPV感染率(34.69%)显著高于对照组(7.50%),差异均有统计学意义(P<0.05)。宫颈癌组LncRNA SNHG12表达水平(2.17±0.55)显著高于CIN组(1.46±0.35)和对照组(1.00±0.31),且CIN组显著高于对照组,差异有统计学意义(P<0.05)。CINⅢ组、CINⅡ组LncRNA SNHG12表达水平显著高于CINⅠ组,差异有统计学意义(P<0.05)。肿瘤低分化、FIGO分期为Ⅲ期的宫颈癌患者癌组织LncRNA SNHG12表达水平显著高于肿瘤中高分化、FIGO分期为Ⅰ、Ⅱ期者,差异有统计学意义(P<0.05),且LncRNA SNHG12表达水平随HPV病毒负荷量增加显著升高。Spearman分析结果显示,LncRNA SNHG12表达水平与HR-HPV感染呈正相关(r=0.357,P<0.05)。多因素Logistic回归分析结果显示,HR-HPV感染、LncRNA SNHG12均是宫颈癌的危险因素(OR=1.761、2.335、2.501、1.876,95%CI:0.941~3.297、1.514~3.601、1.352~4.628、1.440~2.444,P<0.05)。结论宫颈癌组织中LncRNA SNHG12在高表达,与HR-HPV感染密切相关,二者是宫颈癌发生的独立危险因素。

Genes Expressing Differences in Upland Cotton Fiber Development Between 12 DPA and 16 DPA

Cotton is the major dominant natural fiber crop on the earth.Although some current cotton genetics and breeding programs had made great progresses in cotton lint yield increases and disease resistance(tolerance),fiber quality has little improvement.Global understanding genes expression

lncRNA-SNHG12在重度子痫前期患者胎盘组织中的表达及其对滋养细胞增殖的影响

目的探讨长链非编码RNA(lncRNA)小核仁RNA宿主基因12(SNHG12)在重度子痫前期患者胎盘组织中的表达及其对滋养细胞(HTR8/SVneo)增殖的影响。方法采用实时荧光定量PCR(qRT-PCR)检测25例正常产妇(正常组)及25例重度子痫前期患者(sPE组)胎盘组织中lncRNA-SNHG12的表达。将HTR8/SVneo细胞分为3组:过表达组、抑制组和对照组,分别转染pcDNA3.1-SNHG12、siRNA-SNHG12和空质粒。qRT-PCR法检测转染后24 h各组lncRNA-SNHG12、miRNA-30a-3p及其靶基因DNA甲基转移酶3a(DNMT3a)mRNA的表达,蛋白免疫印迹(Western blot)检测DNMT3a蛋白水平的表达。CCK-8法检测转染后24,48,72 h细胞的增殖情况。结果qRT-PCR结果显示,与正常组比较,sPE组胎盘组织中lncRNA-SNHG12的表达量显著降低(P<0.001)。与对照组相比,过表达组lncRNA-SNHG12表达升高,miR-30a-3p的表达降低(P<0.001);抑制组lncRNA-SNHG12表达降低,miR-30a-3p表达增加(P<0.001)。与对照组比较,过表达组DNMT3a mRNA及蛋白水平表达均增加(P<0.001),抑制组DNMT3a mRNA及蛋白水平表达均降低(P<0.001)。CCK-8检测结果显示,与对照组相比较,抑制组24,48,72 h细胞增殖能力均显著降低(P<0.01),过表达组24,48,72 h细胞增殖能力均升高(24 h:P=0.062;48,72 h:P<0.01)。结论lncRNA-SNHG12与子痫前期发病相关,lncRNA-SNHG12可能通过影响miR-30a-3p/DNMT3a途径,调节滋养细胞增殖能力。

基于线粒体12S rRNA基因对大理州亚洲 带绦虫遗传多样性的分析

目的为了解云南省大理州亚洲带绦虫的遗传多样性。方法本研究采集到大理(DL)、巍山(WS)、弥渡(MD)、漾濞(YB)和洱源(EY)5个地区的131份亚洲带绦虫样本,基于线粒体12S rRNA基因进行扩增,运用MEGA7.0和DNASP5.10.01软件对所得序列进行分析,计算其碱基含量、遗传多样性参数、遗传分化系数和基因流以及遗传距离等数据。结果5个地区的亚洲带绦虫12S rRNA基因片段大小均为493 bp,平均A、T、G、C的碱基含量为28.3%、43.2%、19.4%和9.1%;共定义76个单倍体型,其中单倍型多样性为0.9830,核酸多样性为0.0332;遗传分化指数和基因流范围分别为-0.01913~0.04080和5.87745~22.49795;遗传距离为0.0023~0.0229,大理与巍山之间的遗传距离最大,漾濞与洱源群体之间的遗传距离最小。结论大理州5个地区亚洲带绦虫的线粒体12S rRNA基因的遗传多样性水平较高,基因交流频繁,但种群间的遗传分化较弱,本研究为亚洲带绦虫遗传多样性提供了基础数据。