AAV2-PDE6B restores retinal structure and function in the retinal degeneration 10 mouse model of retinitis pigmentosa by promoting phototransduction and inhibiting apoptosis

Retinitis pigmentosa is a group of inherited diseases that lead to retinal degeneration and photoreceptor cell death.However,there is no effective treatment for retinitis pigmentosa caused by PDE6B mutation.Adeno-associated virus(AAV)-mediated gene therapy is a promising strategy for treating retinitis pigmentosa.The aim of this study was to explore the molecular mechanisms by which AAV2-PDE6B rescues retinal function.To do this,we injected retinal degeneration 10(rd10)mice subretinally with AAV2-PDE6B and assessed the therapeutic effects on retinal function and structure using dark-and light-adapted electroretinogram,optical coherence tomography,and immunofluorescence.Data-independent acquisition-mass spectrometry-based proteomic analysis was conducted to investigate protein expression levels and pathway enrichment,and the results from this analysis were verified by real-time polymerase chain reaction and western blotting.AAV2-PDE6B injection significantly upregulated PDE6βexpression,preserved electroretinogram responses,and preserved outer nuclear layer thickness in rd10 mice.Differentially expressed proteins between wild-type and rd10 mice were closely related to visual perception,and treating rd10 mice with AAV2-PDE6B restored differentially expressed protein expression to levels similar to those seen in wild-type mice.Kyoto Encyclopedia of Genes and Genome analysis showed that the differentially expressed proteins whose expression was most significantly altered by AAV2-PDE6B injection were enriched in phototransduction pathways.Furthermore,the phototransductionrelated proteins Pde6α,Rom1,Rho,Aldh1a1,and Rbp1 exhibited opposite expression patterns in rd10 mice with or without AAV2-PDE6B treatment.Finally,Bax/Bcl-2,p-ERK/ERK,and p-c-Fos/c-Fos expression levels decreased in rd10 mice following AAV2-PDE6B treatment.Our data suggest that AAV2-PDE6B-mediated gene therapy promotes phototransduction and inhibits apoptosis by inhibiting the ERK signaling pathway and upregulating Bcl-2/Bax expression in retinitis pigmentosa.

Evaluation of angiotensin converting enzyme insertion/deletion, alpha adducin (ADD1) G460W, and IL-10 gene polymorphisms, and determination of prognostic effects in idiopathic sudden sensorineural hearing loss

Objective:The aim of this study was to examine angiotensin converting enzyme(ACE)insertion/deletion,alpha adducin,and interleukin-10(IL-10)gene polymorphisms(GPs)in terms of both idiopathic sudden sensorineural hearing loss(ISSNHL)risk and their potential prognostic effects.Methods:The study group consisted of 70 patients and the control group consisted of 50 patients.Venous blood samples were analyzed for relevant GPs via kompetitive allele-specific polymerase chain reaction.Age,sex,affected side,tinnitus,and vertiginous symptom status,number of days between symptom onset and hospital admission,pure tone audiometry results at admission and after treatment were included in the study.Data were compared statistically.Results:The D allele of ACE insertion/deletion GP was significantly more frequent in patients with ISSNHL than in the control group(p=0.032).II genotype was associated with a reduced risk of ISSNHL(p=0.036).The amount of hearing loss was significantly higher in patients with the TT genotype(p=0.027)and T allele of the IL-10 GP(p=0.035)than in the patients without this allele.Severe hearing loss was a poor prognostic factor(p=0.008).Conclusions:The D allele of ACE insertion/deletion GP may be involved in the ISSNHL etiology.Due to the association of this allele with occlusive vascular pathologies,ischemia is believed to be a common pathway in the etiopathogenesis of ISSNHL.

vIL-10转基因治疗兔膝关节炎模型的实验研究

目的以逆转录病毒重组体rRV-vIL-10为治疗基因,通过体内外基因转移的动物实验研究,建立局部兔膝关节炎间接体内基因治疗方法。方法①利用可以稳定表达hIL-1β的兔滑膜原代细胞(MFG-hIL-1β-neo-HIG-82)诱导出兔膝关节炎模型。②在体内实验中,将在体外培养的已转染rRV-vIL-10的兔关节滑膜细胞经G418筛选出阳性细胞后回输注入兔膝关节腔内,进行间接体内基因治疗。③通过RT-PCR方法和免疫组化法证实治疗基因转移至体内的滑膜组织并有效表达目的蛋白。④ELISA方法测定关节炎的相关细胞因子在基因治疗前后的水平变化。结果①通过RT-PCR及免疫组化的方法证实逆转录病毒重组体rRV-vIL-10能有效转染兔膝关节的滑膜组织。②应用rRV-vIL-10重组体进行局部间接体内基因治疗可以明显改善hIL-1β诱导的兔膝关节炎模型的关节炎症,下调炎症相关的细胞因子hIL-1β的水平。结论逆转录病毒重组体rRV-vIL-10可以成功地将vIL-10基因导入兔滑膜成纤维样细胞和滑膜组织,明显降低hIL-1β诱导的兔膝关节炎的炎症水平。

携带vIL-10的逆转录病毒重组体的构建及体外表达研究

目的构建携带vIL-10表达序列的重组逆转录病毒rRV-vIL-10并检测该重组病毒对体外培养的兔滑膜细胞的转染情况和目的基因的表达水平。方法①设计带有酶切位点的引物,对含有目的基因的质粒进行PCR扩增并纯化目的基因片段。②双酶切目的基因vIL-10与逆转录病毒载体pLXSN,将pLXSN与vIL-10进行定向克隆连接,筛出阳性克隆并进行鉴定。③扩增逆转录病毒重组体rRV-vIL-10,与辅助质粒pVSVG通过磷酸钙-共沉淀法共转染GP-293包装细胞,收集病毒并测定滴度。④将获得的重组逆转录病毒rRV-vIL-10转染体外培养的兔滑膜成纤维样细胞。细胞免疫组化测定目的蛋白的表达。结果①成功构建了携带治疗基因的重组逆转录病毒rRV-vIL-10,病毒滴度为5×106cfu/ml。②rRV-vIL-10能有效转染体外培养的兔滑膜成纤维样细胞,细胞免疫组化法可检测到vIL-10的表达。结论①成功构建了携带治疗基因vIL-10的重组逆转录病毒rRV-vIL-10。②以逆转录病毒为载体可以成功地将vIL-10基因导入体外培养的兔滑膜成纤维样细胞并表达vIL-10蛋白。

羊口疮病毒疫苗株与野毒株VIL-10基因的比较分析

试验旨在比较分析羊口疮病毒(orf virus,ORFV)VIL-10基因在疫苗株和野毒株之间的差异特征。参照GenBank中公布的ORFV NZ2株的VIL-10基因序列设计并合成1对特异性引物,分别以疫苗株和野毒株提取的基因组DNA为模板,采用PCR方法扩增ORFV的VIL-10基因全序列并进行测序,应用生物信息学相关软件分析基因的核苷酸、氨基酸变异情况及蛋白结构。结果显示,本试验测定的疫苗株和野毒株VIL-10基因核苷酸序列同源性为94.4%,差异主要是单个碱基的突变,其中疫苗株在132~134bp核苷酸序列出现缺失;氨基酸序列同源性为92.5%,出现了15个氨基酸位点的突变,其中疫苗株第42位氨基酸天冬酰胺出现缺失;蛋白质在一级结构及理化性质、二级结构、三级结构、抗原表位参数及有无信号肽之间均存在一定程度的差异,而疫苗株和野毒株编码的蛋白质均无跨膜结构域。系统进化树分析结果表明,本试验测定的野毒株与疫苗株属于不同分支,遗传关系较远。研究结果提示,野毒株与疫苗株的VIL-10基因发生较明显的变异,这些变异可能与ORFV疫苗株的毒力致弱有关。

羊口疮病毒凤翔株ORFV121和vIL-10基因的生物信息学分析

为分析羊口疮病毒ORFV121和vIL-10基因在凤翔(FX0910)强毒株(vORFV)和弱毒株(lvORFV)之间的差异,应用PCR方法扩增羊口疮病毒ORFV121和vIL-10基因的全长序列并测序,应用生物信息学软件分析基因的核酸、氨基酸相似性,蛋白的亲水性、二级结构以及抗原性。结果显示,lvORFV的ORFV121基因118位的谷氨酸缺失,说明该处发生的碱基突变为有意突变,该突变导致弱毒株相应蛋白的亲水性、二级结构发生变化,蛋白的抗原性在很多区域发生本质改变;vIL-10在蛋白质水平出现了5个氨基酸位点突变(14:V→W,49:A→P,57:T→M,72:R→C,102:I→V)和79位插入1个色氨酸。这些位点差异导致蛋白的亲水性、二级结构和抗原性发生了变化。ORFV121基因和vIL-10基因在vORFV和lvORFV之间存在差异,这些基因差异导致蛋白的亲水性、二级结构和抗原性发生改变。

Overexpression of kallikrein gene 10 is a biomarker for predicting poor prognosis in gastric cancer

AIM:To analyze the expression of kallikrein gene 10(KLK10)in gastric cancer and to determine whether KLK10 has independent prognostic value in gastric cancer.METHODS:We studied KLK10 expression in 80 histologically confirmed gastric cancer samples using realtime quantitative reverse transcription-PCR and hK10expression using immunohistochemistry.Correlations with clinicopathological variables(lymph node metastasis,depth of invasion and histology)and with outcomes(disease-free survival and overall survival)during a median follow-up period of 31 mo were assessed.Gastric cancer tissues were then classified as KLK10 positive or negative.RESULTS:KLK10 was found to be highly expressed in 57/80(70%)of gastric cancer samples,while its expression was very low in normal gastric tissues.Positive relationships between KLK10 expression and lymph node metastasis(P=0.048),depth of invasion(P=0.034)and histology(P=0.015)were observed.Univariate survival analysis revealed that gastric cancer patients with positive KLK10 expression had an increased risk for relapse/metastasis and death(P=0.005 and0.002,respectively).Cox multivariate analysis indicated that KLK10 was an independent prognostic indicator of disease-free survival and overall survival in patients with gastric cancer.CONCLUSION:KLK10 expression is an independent biomarker of unfavorable prognosis in patients with gastric cancer.

Comprehensive mutation screening for 10 genes in Chinese patients suffering very early onset inflammatory bowel disease

AIM: To perform sequencing analysis in patients with very early-onset inflammatory bowel disease (VEO-IBD) to determine the genetic basis for VEO-IBD in Chinese pediatric patients. METHODS: A total of 13 Chinese pediatric patients with VEO-IBD were diagnosed from May 2012 and August 2014. The relevant clinical characteristics of these patients were analyzed. Then DNA in the peripheral blood from patients was extracted. Next generation sequencing (NGS) based on an Illumina-Miseq platform was used to analyze the exons in the coding regions of 10 candidate genes: IL-10, IL-10RA, IL-10RB, NOD2, FUT2, IL23R, GPR35, GPR65, TNFSF15, and ADAM30. The Sanger sequencing was used to verify the variations detected in NGS. RESULTS: Out of the 13 pediatric patients, ten were diagnosed with Crohn's disease, and three diagnosed with ulcerative colitis. Mutations in IL-10RA and IL-10RB were detected in five patients. There were four patients who had single nucleotide polymorphisms associated with IBD. Two patients had IL-10RA and FUT2 polymorphisms, and two patients had IL-10RB and FUT2 polymorphisms. Gene variations were not found in the rest four patients. Children with mutations had lower percentile body weight ( 1.0% vs 27.5%, P = 0.002) and hemoglobin ( 87.4 g/L vs 108.5 g/L, P = 0.040) when compared with children without mutations. Although the age of onset was earlier, height was shorter, and the response to treatment was poorer in the mutation group, there was no significant difference in these factors between groups. CONCLUSION: IL-10RA and IL-10RB mutations are common in Chinese children with VEO-IBD. Patients with mutations have an earlier disease onset, lower body weight and hemoglobin, and poorer

miR-10b promotes porcine immature Sertoli cell proliferation by targeting the DAZAP1 gene

MicroRNAs(miRNAs) have been widely identified in porcine testicular tissues and implicated as crucial regulators of proliferation, apoptosis, and differentiation in porcine spermatogenesis related cells. However, the function roles of most of the miRNAs that have been identified in Sertoli cells are poorly understood. In the present study, six experiments were conducted to study the regulatory role of miR-10b in porcine immature Sertoli cells. In experiment 1, the results showed that the relative mRNA expression level of miR-10b in porcine testicular tissues decreased quadratically(P<0.001) with increasing age, while the relative mRNA expression level of DAZAP1 gene increased(P<0.001). In addition, the mRNA expression of miR-10b was negatively(P<0.01) correlated with DAZAP1 mRNA expression(r=–0.550). In experiment 2, the results from the bioinformatic analysis and a luciferase reporter assay demonstrated that miR-10b directly targeted the DAZAP1 gene in porcine immature Sertoli cells. DAZAP1 mRNA and protein expressions were both regulated(P<0.05) by miR-10b. In experiments 3 to 5, the over-expression of miR-10b or the siRNA-mediated knockdown of the DAZAP1 gene promoted(P<0.05) porcine immature Sertoli cell proliferation, as determined by the Cell Counting Kit-8(CCK-8) assay and the 5-Ethynyl-2′-deoxyuridine(EdU) assay. However, an annexin V-FITC/PI staining assay and the expression of cell survival-related genes indicated that over-expression of miR-10b or knockdown of DAZAP1 had no effect(P>0.05) on porcine immature Sertoli cell apoptosis. In experiment 6, the co-transfection treatment results showed that miR-10b promoted(P<0.05) porcine immature Sertoli cell proliferation by targeting DAZAP1 gene. Overall, these experiments demonstrated that miR-10b promotes porcine immature Sertoli cell proliferation by targeting the DAZAP1 gene.

Polymorphisms in interleukin-10 gene according to mutations of NOD2/CARD15 gene and relation to phenotype in Spanish patients with Crohn's disease

AIM： To examine the contribution of interleukin-10 （IL-10） gene polymorphisms to Crohn＇s disease （CD） phenotype, and the possible genetic epistasis between IL-10 gene polymorphisms and CARD15/NOD2 gene mutations. METHODS： A cohort of 205 Spanish unrelated patients with Crohn＇s disease recruited from a single center was studied. All patients were rigorously phenotyped and followed-up for at least 3 years （mean time, 12.5 years）. The clinical phenotype was established prior to genotyping. RESULTS： The correlation of genotype-Vienna classification groups showed that the Ueocolonic location was significantly associated with the -1082G allele in the NOD2/CARD15 mutation-positive patients （RR = 1.52, 95%CI, 1.21 to 1.91,P= 0.008）. The multivariate analysis demonstrated that the IL-10 G14 microsatellite allele in the NOD2/CARD15 mutation positive patients was associated with two risk factors, history of appendectomy （RR = 2.15, 95%CI = 1.1-4.30, P= 0.001） and smoking habit at diagnosis （RR= 1.29, 95%CI= 1.04-4.3, P= 0.04）. CONCLUSION： In Spanish population from Madrid, in CD patients carrying at least one NOD2/CARD15 mutation, the -1082G allele is assodated with ileocolonic disease and the IL-IOG14 microsatellite allele is associated with previous history of appendectomy and smoking habit at diagnosis. These data provide further molecular evidence for a genetic basis of the clinical heterogeneity of CD.

Suppressive Effects of Genomic Imprinted Gene PEG10 on Hydrogen Peroxide-induced Apoptosis in L0_2 Cells

The effects of PEG10 on hydrogen peroxide （H2O2）-induced apoptosis in human normal liver cell line L02 were investigated. The PEG10 gene was transfected into L02 cells by lipofectamine, the positive clone was screened by G418 and defined as L02/PEG10, while the cell transfected with empty expression vector （pEGFP-N1） was defined as L02/vector. L02/vector and parental L02 cells served as control. RT-PCR and Western blotting were employed to detect the expression of target genes. H2O2 （50–400 mmol/L） was administered to induce the apoptosis of L02 cells. Cells viability was measured by MTT and the morphological changes of apoptotic cells were determined by fluorescence microscopy using hoechst33342 nuclei staining. DNA fragmentation was observed by agarose gel electrophoresis. PEG10 mRNA and protein levels in L02/PEG10 cells were significantly increased as compared with those in the control cells. After treatment with 400 mmol/L H2O2 for 24 h, the cellular growth inhibition rate of L02/PEG10 cells was significantly lower （58.2%） than that of L02 （92.5%） and L02/vector （88%）. Distinct morphological changes characteristic of cell apoptosis such as karyopyknosis and conglomeration were not observed in L02/PEG10. Ladder-like DNA fragmentation in a dose-dependent manner was observed in both L02 and L02/vector cell lines, but not in L02/PEG10. PEG10 over-expression significantly inhibited cytotoxicity induced by H2O2 on human normal liver cell line L02 by antagonizing H2O2-induced apoptosis.

Interleukin-10 gene polymorphisms and hepatocellular carcinoma susceptibility:A meta-analysis

AIM: To assess the association between Interleu-kin-10 (IL-10) gene IL-10-1082 (G/A), IL-10-592(C/A), IL-10-819 (T/C) polymorphisms and hepatocellular carcinoma (HCC) susceptibility.METHODS: Two investigators independently searched the Medline, Embase, China National Knowledge Infrastructure, and Chinese Biomedicine Database. Summary odds ratios (ORs) and 95% conf idence intervals (95% CIs) for IL-10 polymorphisms and HCC were cal-culated in a fixed-effects model (the Mantel-Haenszel method) and a random-effects model (the DerSimonian and Laird method) when appropriate. RESULTS: This meta analysis included seven eligiblestudies, which included 1012 HCC cases and 2308 controls. Overall, IL-10-1082 G/A polymorphism was not associated with the risk of HCC (AA vs AG + GG, OR = 1.11, 95% CI = 0.90-1.37). When stratifying for ethnicity, the results were similar (Asian, OR = 1.12, 95% CI = 0.87-1.44; non-Asian, OR = 1.10, 95% CI = 0.75-1.60). In the overall analysis, the IL-10 polymorphism at position -592 (C/A) was identified as a genetic risk factor for HCC among Asians; patients carrying the IL-10-592*C allele had an increased risk of HCC (OR = 1.29, 95% CI = 1.12-1.49). No association was observed between the IL-10-819 T/C polymorphism and HCC susceptibility (TT vs TC + CC, OR = 1.02, 95% CI = 0.79-1.32).CONCLUSION: This meta-analysis suggests that IL-10-592 A/C polymorphism may be associated with HCC among Asians. IL-10-1082 G/A and IL-10-819 T/C polymorphisms were not detected to be related to the risk for HCC.

鱼类白介素10的研究进展

白介素10(IL-10)是能够参与机体免疫的一种多功能细胞因子,由单核细胞、巨噬细胞等多种免疫细胞分泌,在肿瘤、感染、免疫缺陷等多种疾病的发生发展过程中发挥着重要的调节作用。多种硬骨鱼IL-10基因被克隆表达,被证实具有免疫调节作用,目前已有不少关于鱼类IL-10的生物活性、作用机制、调节机制的研究。本文根据已有报道,从鱼类IL-10的基因结构、转录表达、来源与进化、生物学活性及功能、鱼类IL-10受体及信号通路等5个方面进行了综述,为鱼类IL-10的研究与应用提供依据。

IL-1、IL-1β、IL-6、IL-10基因多态性与糖尿病性牙周炎发生的关系分析

目的分析白介素-1(IL-1)、白介素-1β(IL-1β)、白介素-6(IL-6)、白介素-10(IL-10)基因多态性与糖尿病性牙周炎发生的关系。方法选取2021年6月至2022年6月石家庄市第二医院口腔科收治的糖尿病性牙周炎患者60例(观察组)及同期接受口腔检查健康人群60名(对照组)为研究对象,比较两组血清、龈沟液IL-1、IL-1β、IL-6、IL-10表达水平,检测全血DNA中IL-1、IL-1β、IL-6、IL-10基因多态性,分析其与糖尿病性牙周炎易感性的关系。结果观察组血清、龈沟液中IL-1、IL-1β、IL-6、IL-10水平明显高于对照组(t=31.987、28.911、14.201、16.562、21.315、19.146、-45.554、-57.942,P<0.05),各组龈沟液中IL-1、IL-1β、IL-6、IL-10水平明显高于血清中表达,差异有统计学意义(t=-4.080、-10.316、-10.686、10.713;t=-9.567、-6.422、-9.904、3.944,P<0.05)。观察组IL-1基因rs7413228、IL-1β基因rs2356789、IL-6基因rs5357964、IL-10基因rs4543211位点与糖尿病性牙周炎发生相关(P<0.05)。IL-1基因rs7413228位点等位基因T、IL-1β基因rs2356789位点等位基因T、IL-10基因rs4543211位点等位基因G分布频率与糖尿病性牙周炎发生相关(P<0.05)。IL-1基因rs7413228、IL-1β基因rs2356789、IL-6基因rs5357964、IL-10基因rs4543211位点多态性是糖尿病性牙周炎发生的独立影响因素(P<0.05)。结论IL-1、IL-1β、IL-6、IL-10基因多态性与糖尿病性牙周炎易感性相关,临床可通过检验患者基因多态性评估糖尿病性牙周炎发生风险。

SNHG10低表达与卵巢癌预后和耐药的相关性研究

目的:探讨长链非编码小核仁RNA宿主基因10(SNHG10)与卵巢癌细胞增殖、耐药及预后的关系。方法:通过开放大数据(库)筛选88例正常卵巢组织和426例卵巢癌组织中差异表达SNHGs,分析其与卵巢癌患者预后的相关性,并通过受试者工作特征(ROC)曲线评估SNHGs预警卵巢癌紫杉醇和铂类药物耐药的价值。采用实时荧光定量PCR(RT-qPCR)检测SNHG10在卵巢癌紫杉醇/卡铂耐药细胞(SKOV3-R/SKOV3-CBP)及其亲本细胞(SKOV3)中的相对表达水平。通过慢病毒感染在卵巢癌亲本细胞SKOV3中构建过表达SNHG10的细胞株,分为对照组(S-eGFP组)和过表达组(S-SNHG10组)。采用CCK-8、平板克隆形成实验评估细胞增殖能力;通过Cell Titer-Glo发光活细胞检测法评估细胞对紫杉醇的敏感性。结果:SNHG10在卵巢癌组织显著低表达(P<0.01),其低表达与卵巢癌患者不良预后显著相关(P<0.05),且能潜在预测紫杉醇和铂类化疗耐药(AUC>0.6,P<0.05)。与S-eGFP组相比,S-SNHG10组细胞的增殖能力下降,对紫杉醇的敏感性增强(P<0.001)。结论:过表达SNHG10显著抑制卵巢癌细胞增殖并提高卵巢癌细胞对紫杉醇的敏感性。

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.

Production of homeobox A10 gene transgenic pigs by somatic cell nuclear transfer

Homeobox A10(Hoxa10) gene is one of the most important candidate genes associated with the reproductive performance of humans and mice. Overexpression of Hoxa10 in mouse endometrium can increase litter size. Moreover, Hoxa10 plays a key role in regulating the embryo implantation of sows. This study aimed to generate transgenic pigs using Hoxa10 via somatic cell nuclear transfer(SCNT). We established seven Hoxa10-transgenic cell lines, and two of the cell lines were selected as nuclear donors for the transfer. A total of 1 270 cloned embryos were generated and transferred to five surrogate mothers(Landrace×Yorkshire). Eight cloned male piglets were produced including one with cryptorchidism. Six transgenic piglets grew up healthy and produced 56 offspring. Finally, we obtained six transgenic male pigs and 26 transgenic positive offspring that can be used to further study the regulatory mechanism of Hoxa10 on the reproductive performance of pigs.

Construction of Eukaryotic Expression Vector of Human CC10 Gene and Expression of CC10 Protein in Lung Adenocarcinoma A549 Cell Line

Summary： A mammalian expression plasmid pcDNA3. 1-hCC10 was constructed and identified, then CC10 protein expression in A549 lung cancer cell line was detected. A 273 bp cDNA fragment was amplified from the total RNA of normal lung tissue by using RT-PCR and cloned into expression plasmid cDNA3. 1, and the recombinant plasmid was identified by employing double digestion restriction enzymes HindⅢ and BanH 1 and the cDNA sequence was assayed by the Sanger dideoxymediated chain termination method. The segment was then transfected into the A549 lung cancer cell line. The protein expression of CC10 was detected by immunofluorescence and Western blot. Our results showed that the cDNA fragment included the entire coding region （273 bp）. The re combinant eukaryotic cell expression vector of pcDNA3. 1-hCC10 was successfully constructed, and the sequence of the insert was identical to the published sequence. A549 cells line transfected with the pcDNA3. 1-hCC10 expressed high level of CC10 protein. The recombinant plasmid cDNA3. 1- hCC10 may serve as an effecnve tool for the study of tumorogenesis and tumor treatment.

白细胞介素10受体A基因突变导致的极早发型炎症性肠病临床特点及基因分析

目的总结白细胞介素10受体A(interleukin 10 receptor A,IL-10RA)基因突变导致的极早发型炎症性肠病(very early onset inflammatory bowel disease,VEO-IBD)患儿临床特点和遗传学特征。方法回顾性分析2007年3月到2019年5月在首都医科大学附属北京儿童医院院消化科住院的慢性腹泻的患儿中,确诊为VEO-IBD的患儿,其中病因为IL-10RA基因突变的患儿15例,对照组为15例非IL-10RA突变所致VEO-IBD患儿,统计分析其临床特点及基因报告。结果IL-10RA基因突变所致的VEO-IBD患儿,克罗恩病(Crohn s disease,CD)11例,溃疡性结肠炎(ulcerative colitis,UC)4例,临床症状以慢性腹泻(15/15例,100.0%)、便血(15/15例,100.0%)为主,肠外表现依次为口腔黏膜溃疡(6/15例,40.0%)、皮肤红斑(5/15例,33.3%);肛周表现依次为直肠会阴瘘5例(5/15,33.3%),肛瘘4例(4/15,26.7%),肛裂3例(3/15,20.0%),直肠会阴瘘、皮赘并存1例(1/15,6.7%);全身表现为IL-10RA基因突变组营养不良13例(13/15例,86.7%),肛周病变13例(13/15例,86.7%);对照组营养不良6例(6/15例,40.0%),肛周病变5例(5/15例,33.3%),此两项指标与IL-10RA基因突变组相比,差异有统计学意义(P<0.05)。15例IL-10RA突变患儿中,共检测到9个突变位点,其中c.301c>T(p.R101W)和c.537G>A(p.T179T)为最常见的突变位点。IL-10RA突变导致炎症因子增高,引起肠道炎症反应。凝血酶原时间和部分凝血活酶时间均明显延长。结论IL-10RA基因突变导致的VEO-IBD患儿发病年龄早,除消化道症状外,肠外表现和肛周病变较为常见,结肠镜下病变特点以结肠多发溃疡最常见,其次为炎性息肉。c.301c>T(p.R101W)和c.537G>A(p.T179T)为最常见的基因突变位点。IL-10RA突变导致炎症因子增高,引起肠道炎症反应。

1株血清10型副猪嗜血杆菌的分离鉴定与生物学特性分析

【目的】阐明引起荆州某猪厂仔猪疑似副猪嗜血杆菌病的病原生理生化特性、毒力与药物敏感性,为今后对该病的防治提供科学依据。【方法】从患病仔猪中分离培养病原菌,通过形态学观察、生理生化鉴定、PCR鉴定、16S rRNA基因测序、血清型鉴定、多序列位点分型(MLST)对分离菌株进行鉴定。通过毒力基因检测、小鼠致病性、药敏试验、中药治疗试验等对分离株进行致病性、耐药性分析。【结果】通过形态学观察、生理生化试验、16S rRNA序列比对、系统进化树分析确定分离菌株为副猪嗜血杆菌。通过血清型与MLST分析确定分离菌株为血清10型、ST型为299。毒力基因检测发现,分离菌株具有CapD、vta 1、vta 2等15种毒力基因。将分离菌株腹腔注射感染小鼠,可导致小鼠多个脏器发生明显病变,具有较强致病性。耐药基因检测试验发现,分离菌株具有β-内酰胺类耐药基因bla OXA和氟喹诺酮类耐药基因gyrA。药敏试验结果显示,分离菌株对头孢他啶、新霉素、米诺环素等10种抗菌药物敏感,同时对明雄黄、款冬花、全蝎3种中药敏感。中药治疗试验结果表明,明雄黄和全蝎对分离菌株感染小鼠有较明显的治疗作用。【结论】试验成功分离1株血清10型副猪嗜血杆菌,侵染小鼠可致多个器官出血坏死,该菌株对10种抗菌药物及3种中药敏感,且明雄黄和全蝎对分离菌株感染小鼠治疗效果明显。研究结果可为今后副猪嗜血杆菌的防治和临床诊疗提供参考依据。