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Hepatitis B virus upregulates host expression of α-1,2-mannosidases via the PPARα pathway 被引量:3
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作者 Song Hu Li-Bin Jiang +2 位作者 Xiao-Jing Zou Wei Yi De-Ying Tian 《World Journal of Gastroenterology》 SCIE CAS 2016年第43期9534-9543,共10页
AIM To assess the effects of hepatitis B virus(HBV) on the expression of host α-1,2-mannosidases and determine the underlying mechanisms.METHODS We measured the expression levels of MAN1A1, MAN1A2, MAN1B1, and MAN1C1... AIM To assess the effects of hepatitis B virus(HBV) on the expression of host α-1,2-mannosidases and determine the underlying mechanisms.METHODS We measured the expression levels of MAN1A1, MAN1A2, MAN1B1, and MAN1C1 in cell lines HepG 2.2.15, HepN 10, HepA D38 and Hep G2 by Western blot. Viral antigens(HBs Ag and HBe Ag) in the culture medium were measured using the chemiluminescence method. HBV DNA quantification assays were performed using a commercial real-time PCR kit. Protein levels of human liver tissue α-1,2-mannosidases were also evaluated by Western blot. Plasmids containing seven individual viral genes of HBV(PTT22-HBx, PTT22-HBs, PTT22-pre S2, PTT22-pre S1, PTT22-HBc, PTT22-HBe, and PTT22-HBp) or control plasmids(PTT22-vector) were transfected into Hep G2 cells. MK886(PPARα) and GW9662(PPARγ) inhibitors were used to explore the effects of HBV on α-1,2-mannosidase expression after the PPARα and PPARγ pathways were blocked.RESULTS We showed that the expression of α-1,2-mannosidases was higher in stably transfected HBV cells than in controls. The expression levels of α-1,2-mannosidase were higher in AD38 cells than those in ND10 cells, which were in turn greater than those in G2.2.15 cells, and positively correlated with the expression of HBsA gin all the cell lines. Levels of α-1,2-mannosidase in nontumorous liver tissues of HBV-related HCC patients were also higher than in the tissues from non-HBVrelated HCC patients. Moreover, transfecting Hep G2 cells with a component of the HBV viral envelope also increased the expression of α-1,2-mannosidases. However, this envelope protein component could not induce MAN1C1 expression in the presence of a PPARα inhibitor, MK886. We also found that MK886 did not affect the expression of MAN1C1 in AD38 cells without tetracycline in the culture medium. This phenomenon was not observed in the case of GW9662.CONCLUSION Our results indicate that HBV increases the expression of α-mannosidases both in vitro and in vivo via activation of the PPARα pathway by its envelope protein. 展开更多
关键词 肝炎 B 模式识别受体 α -mannosidase GLYCOSYLATION 树枝状的房间
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Effect of Oxytropis glabra DC. Poisoning on α-Mannosidase(AMA) Expression in Mice Brain Tissue
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作者 Wang Shuai Jia Qizhen +2 位作者 Zhang Ling Chen Genyuan Ma Chunhui 《Animal Husbandry and Feed Science》 CAS 2015年第6期366-369,共4页
The effect of Oxytropis glabra DC. on α-mannosidase( AMA) expression in mice brain tissue was explored to reveal the toxicity mechanism of O. glabra. Forty mice were randomly divided into four groups,namely control g... The effect of Oxytropis glabra DC. on α-mannosidase( AMA) expression in mice brain tissue was explored to reveal the toxicity mechanism of O. glabra. Forty mice were randomly divided into four groups,namely control group,experimental group I,experimental group II and experimental group III. The mice in three experimental groups were fed with O. glabra at the doses of 1,5 and 10 g per kilogram weight,respectively. After challenge for 63 d,mice brains were collected to detect changes in distribution and expression of AMA in different brain regions. The results showed that O. glabra poisoning led to declined AMA mRNA expression in mice brain tissue,but the mice in experimental group I had no significant difference with those in control group( P > 0. 05). The AMA mRNA expression in cerebellum,cerebrum and thalamus of mice in experimental groups II and III were significantly lower than that in control group( P < 0. 05),but the AMA mRNA expression in hippocampus and brainstem in three experimental groups had no significant difference with that in control group( P > 0. 05). AMA had very weak expression in hippocampus and brainstem,but it had expressions in other regions,and the expression was positively correlated with the number of neurons and granulosa cells. The results showed that different doses of O. glabra reduced AMA mRNA expression in mice brain tissue,while cerebellum,cerebrum and thalamus were the main target function areas. 展开更多
关键词 Oxytropis glabra α-mannosidase(AMA) POISONING MICE
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英语元音弱化的-man与汉语指人类后缀比较分析
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作者 韦伟韫 《海外英语》 2024年第2期74-77,共4页
-man作为一种构词要素,在英语中大量存在。-man的读音主要有三种类型,第一类是与自由词素相同的完全元音[mæn],如superman[′suːpəmæn];第二类为弱化元音[mən],如postman[′pəʊstmən];第三类读音则在前面两种读音间变化,如fre... -man作为一种构词要素,在英语中大量存在。-man的读音主要有三种类型,第一类是与自由词素相同的完全元音[mæn],如superman[′suːpəmæn];第二类为弱化元音[mən],如postman[′pəʊstmən];第三类读音则在前面两种读音间变化,如freeman[′friːmən]或[′friːmæn]。文章将以元音弱化的-man词汇为研究对象,通过与汉语指人类后缀进行对比分析来判定-man的构词地位。研究发现,元音弱化的-man可以称之为类后缀,其与汉语指人类后缀具有共同特点:1)经历语法化;2)构词稳定;3)具有能产性。 展开更多
关键词 元音弱化的-man 指人类后缀 构式 能产性
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基于CRISPR/Cas9加工番茄α-Man突变体的构建 被引量:5
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作者 张圆圆 邵冬南 崔百明 《生物技术通报》 CAS CSCD 北大核心 2019年第6期9-15,共7页
为培育成熟果实软化程度低,货架期长的番茄植株,以加工番茄甘露糖苷酶基因(α-Man)为编辑对象,设计由番茄U6 启动子驱动、长21 bp 的guide RNA(gRNA)指导hCas9 核酸酶,靶向编辑α-Man 的第1 个外显子。首先构建基于CRISPR/Cas9 系统的... 为培育成熟果实软化程度低,货架期长的番茄植株,以加工番茄甘露糖苷酶基因(α-Man)为编辑对象,设计由番茄U6 启动子驱动、长21 bp 的guide RNA(gRNA)指导hCas9 核酸酶,靶向编辑α-Man 的第1 个外显子。首先构建基于CRISPR/Cas9 系统的植物表达载体,并通过农杆菌介导的遗传转化获得加工番茄转基因株系,然后取转基因番茄叶片基因组DNA,利用限制性内切酶法结合PCR 扩增对α-Man 编辑位点附近的DNA 片段进行检测及测序分析。结果表明,14 株转基因番茄植株有2 株检测到突变现象。α-Man 突变体TA 克隆测序结果显示有2 种编辑类型,一种表现为52 bp 的缺失突变;另一种表现为单碱基突变。实现了对番茄α-Man 的编辑。 展开更多
关键词 加工番茄 CRISPR/Cas9 α-man 果实成熟软化
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Trimming of N-Glycans by the Golgi-Localized α-1,2-Mannosidases, MNS1 and MNS2, Is Crucial for Maintaining RSW2 Protein Abundance during Salt Stress in Arabidopsis 被引量:3
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作者 Chuanfa Liu Guanting Niu +7 位作者 Huchen Zhang Yafei Sun Shubin Sun Fugen Yu Shan Lu Yonghua Yang Jianming Li Zhi Hong 《Molecular Plant》 SCIE CAS CSCD 2018年第5期678-690,共13页
Asparagine (Asn/N)-Iinked glycans are important for protein folding, trafficking, and endoplasmic reticulum-associated degradation in eukaryotes. The maturation of glycoproteins involves the trimming of mannosyl res... Asparagine (Asn/N)-Iinked glycans are important for protein folding, trafficking, and endoplasmic reticulum-associated degradation in eukaryotes. The maturation of glycoproteins involves the trimming of mannosyl residues by mannosidases and addition of other sugar molecules to three-branched N-glycans in the Golgi. However, the biological importance of Golgi-mediated mannose trimming is not fully understood. Here, we show that abolishment of two functionally redundant mannosidases, MNS1 and MNS2, responsible for α-1,2-mannose trimming on the A and C branches of plant N-glycans lead to severe root growth inhibition under salt stress conditions in Arabidopsis. In contrast, mutants with defects in the biosynthesis of the oligosaccharide precursor displayed enhanced salt tolerance in the absence of mannose trimming. However, mutation in EBS3, which is required for the formation of the branched N-glycan precursor, suppressed the salt-sensitive phenotype of mnsl mns2 double mutant. Interestingly, we observed that cellulose biosynthesis was compromised in mnsl mns2 roots under high salinity. Consistently, abundance of a membrane anchored endo-13-1,4-endoglucanase (RSW2/KOR) that plays a key role in cellulose biosynthesis and its mutant variant rsw2-1 were modulated by α-1,2-mannose trimming under salt stress. Overexpression of RSW2 could partially rescue the salt-sensitive phenotype of mnsl mns2. Taken together, these results suggest that MNS1/2-mediated mannose trimming of N-glycans is crucial in modulating glycoprotein abundance to withstand salt stress in plants. 展开更多
关键词 N-GLYCAN Golgi α-mannosidase I salt tolerance ARABIDOPSIS
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Changes in Activities of Three Enzymes Degrading Galactomannan During and Following Rice Seed Germination 被引量:4
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作者 REN Yan-fang HE Jun-yu WANG Xiao-feng 《Rice science》 SCIE 2007年第4期295-301,共7页
To investigate the relationships among β-mannanase, β-mannosidase and a-galactosidase required for degrading galactomannan in cell wall during and following rice seed germination, the activities of the three enzymes... To investigate the relationships among β-mannanase, β-mannosidase and a-galactosidase required for degrading galactomannan in cell wall during and following rice seed germination, the activities of the three enzymes and the effects of ABA and GA3 on them were surveyed. The activities of β-mannosidase and a-galactosidase presented in dry and pre-germinated rice seeds, and increased slowly during and following germination. However, the activity of β-mannanase was detected only after germination. GA3 could promote the activities of β-mannanase and a-galactosidase. ABA had little effect on the activities of β-mannosidase and α-galactosidase, but it could seriously inhibit the activity of β-mannanase. 展开更多
关键词 GERMINATION Β-manNANASE β-mannosidase Α-GALACTOSIDASE enzyme activity rice
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真核生物α-甘露糖苷酶生物信息学分析 被引量:1
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作者 王铎 孙春玉 +1 位作者 陈静 王义 《生命科学研究》 CAS CSCD 2018年第3期173-183,共11页
α-甘露糖苷酶(α-mannosidase,α-Man)是真核生物蛋白质N-聚糖修饰的关键酶,其对甘露糖残基的修剪过程是糖蛋白N-糖链复杂化的必要步骤,对蛋白质的合成及正确构象的折叠起决定性作用。根据α-Man的功能特异性,其一般被分为糖基水解酶3... α-甘露糖苷酶(α-mannosidase,α-Man)是真核生物蛋白质N-聚糖修饰的关键酶,其对甘露糖残基的修剪过程是糖蛋白N-糖链复杂化的必要步骤,对蛋白质的合成及正确构象的折叠起决定性作用。根据α-Man的功能特异性,其一般被分为糖基水解酶38家族(glycosyl hydrolase 38 family,GH38)、糖基水解酶47家族(glycosyl hydrolase 47 family,GH47)两个家族。利用生物信息学分析GH38家族与GH47家族在进化上的关系和氨基酸序列保守性以及不同物种内质网Ⅰ型甘露糖苷酶(endoplasmic reticulum ManⅠ,ERManⅠ)的理化性质、结构特点、功能特征后发现,GH47家族比GH38家族在进化上更早且保守性更好;α-Man基因在不同物种中长度存在明显差异,物种越高等基因平均长度越长;真核生物ERManⅠ均为亲水性不稳定蛋白质,其氨基酸序列存在跨膜螺旋并含有信号肽,且蛋白质空间构像为桶状,包含Ca^(2+)结合位点。文中对α-Man的生物信息学分析可以为研究α-Man在生命过程中的作用提供重要的信息。 展开更多
关键词 α-甘露糖苷酶(α-man) 糖基水解酶38家族(GH38) 糖基水解酶47家族(GH47) 内质网Ⅰ型α-甘露糖苷酶(ERManⅠ) 生物信息学
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浅析对供应商4M变更的规范管理 被引量:3
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作者 张龙刚 《汽车实用技术》 2017年第18期251-253,共3页
随着顾客对产品的个性化需求越来越细化,为了适应这种市场化的要求,大型企业一方面需要遵循严格的产品规范要求,同时又需要对市场变化做出迅速反应,满足不同客户的需求。产品多样小批量的生产变化对提供产品服务的企业运营提出了很大的... 随着顾客对产品的个性化需求越来越细化,为了适应这种市场化的要求,大型企业一方面需要遵循严格的产品规范要求,同时又需要对市场变化做出迅速反应,满足不同客户的需求。产品多样小批量的生产变化对提供产品服务的企业运营提出了很大的挑战,同时对管控产品质量的风险加大。文章通过研究对供应商4M变更管理规范的要求,探讨企业在实际生产过程中针对供应商4M变更的规范管理,有效防范供应商产品4M变更的风险,使企业在当前的生产模式中竞争地位不断增强。 展开更多
关键词 4M(人-man、机-Machine、料-Material、法-Method) 4M变更 供应商管理 质量管理
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Directional screening and identification of potential cytotoxic components from Achnatherum inebrians by a combination of surface palsmon resonance and chromatography
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作者 Wenbin Zhou Man Wang +3 位作者 Aiqin Zhang Danrong Huang Hua Guo Gangyi Shen 《Chinese Herbal Medicines》 CAS 2023年第2期329-336,共8页
Objective:To establish a method for directional screening of the cytotoxic components from the medicinal herb of Achnatherum inebrians by a combination of surface plasmon resonance(SPR)biosensor and chromatographic is... Objective:To establish a method for directional screening of the cytotoxic components from the medicinal herb of Achnatherum inebrians by a combination of surface plasmon resonance(SPR)biosensor and chromatographic isolation technology.Methods:Under the guidance of bioactive assessment based on binding abilities between objects and the a-Mannosidase(a-Man)target,the active components from different solvents extracts,different polar extraction parts and fractions were screened orderly and directionally using SPR.Components with a high binding ability to a-Man can be precisely oriented in a narrower fractions range and are easy to isolate.Three human cancer cells were used to evaluate the cytotoxic activity of component with the highest affinity to a-Man.Results:Eight compounds were isolated and identificated from A.inebrians for the first time.Deoxyvasicinone possessed the highest affinity to a-Man among them.Moreover,deoxyvasicinone showed good effects on inhibited proliferation of human hepatoma cells HepG2(IC_(50)=5.7 μmol/L),human breast cancer cells MCF7(IC_(50)=7.21 μmol/L)and human lung cancer cells HCC827(IC_(50)=0.75 μmol/L),respectively.In particular,its inhibitory effect on HCC827 was stronger than the positive drug gefitinib(IC_(50)=1.65 μmol/L).Conclusion:A comprehensive strategy of directional screening potential cytotoxic components from herb based on biomolecular interaction and chromatography was established.Deoxyvasicinone as an effective anti-cancer component was initially isolated from A.inebrians.It is expected that this screening strategy could provide new perspectives for rapid screening and identification of active components from natural plants with the complex matrix. 展开更多
关键词 Achnatherum inebrians(Hance)Keng CHROMATOGRAPHY cytotoxic components deoxyvasicinone surface plasmon resonance α-mannosidase
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Inhibition of metastasis to lung of a human nasopharyngeal carcinoma cell line CNE-2L2 transfected with pRc/CMV-antisense 6A8 cDNA in nude mice
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作者 张立新 刘玉琴 +10 位作者 马凤蓉 顾蓓 史耕先 赵雪梅 李波 高进 赵方萄 张淑珍 李国燕 王讯 朱立平 《Science China(Life Sciences)》 SCIE CAS 1999年第2期209-215,共7页
The growth of CNE-2L2 cell, a cloned line of human nasopharyngeal carcinoma with a high potentiality of metastasis to lung was inhibited to a certain extent after transfection with a recombinant antisense expression v... The growth of CNE-2L2 cell, a cloned line of human nasopharyngeal carcinoma with a high potentiality of metastasis to lung was inhibited to a certain extent after transfection with a recombinant antisense expression vector of a cDNA encoding a human α-mannosidase (pRc/CMV-antisense 6A8 cDNA)( the Genbank accession number of 6A8 cDNA is U37248) in comparison with that of the cell transfected with the Mock and of the wild cell. Two months after a subcutaneous inoculation of CNE-2L2 cell into the axilla of nude mice metastatic lesions in the lung were observed in 9/10 mice (90%) with grade Ⅲ in 8 mice and grade Ⅱ in one mouse in the wild cell group, in 6/8 mice (75%) with grade Ⅲ in one mouse, grade Ⅱ in 2 mice and grade Ⅰ in 3 mice in the Mock-transfection group, in only 3/10 mice (30%) with all grade Ⅰ in pRc/CMV-antisense 6A8 cDNA-transfection group. 展开更多
关键词 ANTISENSE 6A8 CDNA transfection METASTASIS NASOPHARYNGEAL carcinoma cell line α-mannosidase.
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