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Solid-state NMR of the retinal protonated Schiff base in microbial rhodopsins
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作者 Sari Kumagai Izuru Kawamura 《Magnetic Resonance Letters》 2024年第3期11-18,共8页
Rhodopsin is a seven-helical transmembrane protein with a retinal chromophore covalently bound to a conserved lysine in helix G via a retinal protonated Schiff base(RPSB).Microbial rhodopsins absorb light through chro... Rhodopsin is a seven-helical transmembrane protein with a retinal chromophore covalently bound to a conserved lysine in helix G via a retinal protonated Schiff base(RPSB).Microbial rhodopsins absorb light through chromophore and play a fundamental role in optogenetics.Numerous microbial rhodopsins have been discovered,contributing to diverse functions and colors.Solid-state NMR spectroscopy has been instrumental in elucidating the conformation of chromophores and the three-dimensional structure of microbial rhodopsins.This review focuses on the 15N chemical shift values of RPSB and summarizes recent progress in the field.We displayed the correlation between the 15N isotropic chemical shift values of RPSB and the maximum absorption wavelength of rhodopsin using solid-state NMR spectroscopy. 展开更多
关键词 Membrane proteins Microbial rhodopsin RETINAL Solid-state NMR Protonated Schiff base
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普通大蓟马MuRhodopsin基因的全长克隆及生物信息学分析 被引量:1
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作者 金海峰 王朝政 +3 位作者 侯清芳 咸利民 张华剑 吴少英 《热带生物学报》 2023年第6期651-659,共9页
为了解蓟马害虫视蛋白分子结构及特征,根据普通大蓟马(Megalurothrips usitatus)转录组信息克隆获得了视紫红质MuRhodopsin的基因cDNA全长,并利用DNAMan 9.0和SWISSMODEL等软件对视紫红质MuRhodopsin的基因进行序列同源性比对并构建基... 为了解蓟马害虫视蛋白分子结构及特征,根据普通大蓟马(Megalurothrips usitatus)转录组信息克隆获得了视紫红质MuRhodopsin的基因cDNA全长,并利用DNAMan 9.0和SWISSMODEL等软件对视紫红质MuRhodopsin的基因进行序列同源性比对并构建基因系统进化树,分析理化性质及结合域特点,并对该蛋白进行结构预测。结果表明:该基因全长1140 bp,共编码380个氨基酸,相对分子质量为42.73 kDa,理论等电点为8.47。序列比对以及同源性分析结果表明,MuRhodopsin为横纹视紫红质(rhabdomeric opsins,r-opsins)与西花蓟马(Frankliniella occidentalis)及棕榈蓟马(Thrips palmi)具有高度同源性。结构域分析表明该蛋白具有7个跨膜结构域,包含了1个G蛋白偶联受体家族区域,隶属于G蛋白偶联受体家族;具有6个N-豆蔻酰化位点,3个N-糖基化位点,3个酪蛋白激酶Ⅱ磷酸化位点,4个蛋白激酶C磷酸化位点;其第322位氨基酸—赖氨酸(K)为与发色团(视黄醛)的重要结合位点,具有典型的视蛋白能够激活IP3/Ca2+信号通路引起光依赖的去极化反应。 展开更多
关键词 普通大蓟马 rhodopsin基因 视蛋白 序列分析 结构预测
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Rhodopsin和S-opsin在MNU诱导的大鼠视网膜损伤过程中的表达变化 被引量:1
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作者 高杨 邓新国 李娜 《中国病理生理杂志》 CAS CSCD 北大核心 2010年第12期2428-2432,共5页
目的:观察在N-甲基-N亚硝酸脲(MNU)诱导的大鼠视网膜外核层细胞损伤过程中视紫质(rhodopsin)和蓝光视蛋白(blue-sensitive opsin/S-opsin)在视网膜中的表达变化,分析其与MNU诱导的视网膜损伤的关系。方法:将30只SPF级50 d龄雌性SD大鼠... 目的:观察在N-甲基-N亚硝酸脲(MNU)诱导的大鼠视网膜外核层细胞损伤过程中视紫质(rhodopsin)和蓝光视蛋白(blue-sensitive opsin/S-opsin)在视网膜中的表达变化,分析其与MNU诱导的视网膜损伤的关系。方法:将30只SPF级50 d龄雌性SD大鼠随机分为正常对照组和MNU模型1、3、7、10 d组,每组各6只大鼠。模型组以腹腔注射MNU(40 mg/kg)建立MNU模型;正常对照组大鼠腹腔注射生理盐水(5 mL/kg)。右眼冰冻切片行苏木素-伊红(HE)染色判断视网膜损伤程度。通过逆转录-聚合酶链反应(RT-PCR)和免疫荧光检测各组视网膜中rhodopsin和S-opsin的mRNA及蛋白表达情况。结果:病理检测确定造模结果与以往实验一致,各组病理分级之间的差异显著(2=16.838,P<0.01)。RT-PCR检测结果表明,与正常对照组相比,各MNU模型组rhodopsin和S-opsin的mRNA表达水平随MNU作用时间增加而逐渐降低且差异均显著(rhodopsin 1 d组P<0.05;S-opsin 1 d组P<0.01;3、7、10 d组rhodopsin和S-opsin均P<0.01)。免疫荧光检测结果显示,在正常大鼠视网膜rhodopsin主要在光感受器细胞外段表达,MNU作用后rhodopsin主要在外核层表达,少量在内核层表达,并随MNU作用时间增加而逐渐表达降低。S-opsin在正常视网膜各层均有表达,在各模型组随MNU作用时间增加S-opsin的表达逐渐降低,在外核层和光感受器细胞内、外段尤为明显。结论:MNU诱导的视网膜外核层细胞损伤可降低rhodopsin和S-opsin的表达,并与MNU选择性引起光感受器细胞丧失有关。 展开更多
关键词 N-甲基-N-亚硝酸脲 SD大鼠 视网膜 视紫质 视蛋白
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A COMPLETE SCREEN FOR MUTATIONS OF THE RHODOPSIN GENE IN A PANEL OF CHINESE PATIENTS WITH AUTOSOMAL DOMINANT RETINITIS PIGMENTOSA 被引量:7
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作者 Xiao-liZhang MingLiu +4 位作者 Xiao-hongMeng Wei-lingFu Zheng-qinYin XueZhang Jun-fuHuang 《Chinese Medical Sciences Journal》 CAS CSCD 2005年第1期30-34, ,共5页
Objective To evaluate the prevalence of rhodopsin (RHO) mutations and the genotype-phenotype relationships in Chinese patients with autosomal dominant retinitis pigmentosa (ADRP) by conformation sensitive gel electrop... Objective To evaluate the prevalence of rhodopsin (RHO) mutations and the genotype-phenotype relationships in Chinese patients with autosomal dominant retinitis pigmentosa (ADRP) by conformation sensitive gel electrophoresis (CSGE) and direct DNA sequencing. Methods We have screened the five coding exons and splice sites of RHO gene in 27 probands who had no relativity from Chinese ADRP families and 100 normal controls to identify disease-associated mutations, using CSGE and direct DNA sequencing. Family members of some probands with disease-associated mutations were also genotyped to determine whether the RHO mutations segregated with retinitis pigmentosa (RP) in their families. Results Two RHO mutations, Pro347Leu and Pro327 (1-bp del), were identified separately in two families, thus the frequency of RHO mutations among this set of Chinese ADRP families is about 7.4% (2/27). Pro347Leu mutation was found in one ADRP proband as well as three her children who also had RP. She had relatively early onset at about 17 years. The only one child without this mutation had no symptom or sign of RP at age of 34. Pro327 (1-bp del) was identified in a late-onset ADRP patient, who appeared night blindness around 30 years old and in her fifties electroretinogram (ERG) has been flat in both scotopic and photopic phases. Family analysis showed that this mutation also existed in her younger dau-ghter and her elder sister, both of them also had RP. Three other family members were genotypically and phenotypically normal. Neither of the two mutations was detected in 100 normal controls.Conclusions The frequency of RHO mutations in Chinese patients was lower than that in Europe and North America. The phenotype of the patients with Pro347Leu corresponded to type 1 ADRP, with severe rod degeneration and some cone preservation later, while the phenotype of the patients carrying Pro327 (1-bp del) corresponded to type 2 ADRP, with a concomitant loss of rod and cone visual function. CSGE was found to be a sensitive, simple, and practical method for the screening of a large number of samples under highly reproducible conditions, and could be utilized in routine molecular diagnostic laboratories. 展开更多
关键词 autosomal dominant retinitis pigmentosa rhodopsin mutation conformation sensitive gel electrophoresis
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Binding of rhodopsin and rhodopsin analogues to transducin, rhodopsin kinase and arrestin-1
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作者 Nelson A Araujo Carlos E Sanz-Rodríguez José Bubis 《World Journal of Biological Chemistry》 CAS 2014年第2期254-268,共15页
AIM: To investigate the interaction of reconstituted rhodopsin, 9-cis-retinal-rhodopsin and 13-cis-retinal-rhodopsin with transducin, rhodopsin kinase and arrestin-1. METHODS: Rod outer segments(ROS) were isolated fro... AIM: To investigate the interaction of reconstituted rhodopsin, 9-cis-retinal-rhodopsin and 13-cis-retinal-rhodopsin with transducin, rhodopsin kinase and arrestin-1. METHODS: Rod outer segments(ROS) were isolated from bovine retinas. Following bleaching of ROS membranes with hydroxylamine, rhodopsin and rhodopsin analogues were generated with the different retinal isomers and the concentration of the reconstituted pigments was calculated from their UV/visible absorption spectra. Transducin and arrestin-1 were purified to homogeneity by column chromatography, and an enriched-fraction of rhodopsin kinase was obtainedby extracting freshly prepared ROS in the dark. The guanine nucleotide binding activity of transducin was determined by Millipore filtration using β,γ-imido-(3H)-guanosine 5'-triphosphate. Recognition of the reconstituted pigments by rhodopsin kinase was determined by autoradiography following incubation of ROS membranes containing the various regenerated pigments with partially purified rhodopsin kinase in the presence of(γ-32P) ATP. Binding of arrestin-1 to the various pigments in ROS membranes was determined by a sedimentation assay analyzed by sodium dodecyl sulphatepolyacrylamide gel electrophoresis. RESULTS: Reconstituted rhodopsin and rhodopsin analogues containing 9-cis-retinal and 13-cis-retinal rendered an absorption spectrum showing a maximum peak at 498 nm, 486 nm and about 467 nm, respectively, in the dark; which was shifted to 380 nm, 404 nm and about 425 nm, respectively, after illumination. The percentage of reconstitution of rhodopsin and the rhodopsin analogues containing 9-cis-retinal and 13-cis-retinal was estimated to be 88%, 81% and 24%, respectively. Although only residual activation of transducin was observed in the dark when reconstituted rhodopsin and 9-cis-retinal-rhodopsin was used, the rhodopsin analogue containing the 13-cis isomer of retinal was capable of activating transducin independently of light. Moreover, only a basal amount of the reconstituted rhodopsin and 9-cis-retinal-rhodopsin was phosphorylated by rhodopsin kinase in the dark, whereas the pigment containing the 13-cis-retinal was highly phosphorylated by rhodopsin kinase even in the dark. In addition, arrestin-1 was incubated with rhodopsin, 9-cis-retinal-rhodopsin or 13-cis-retinal-rhodopsin. Experiments were performed using both phosphorylated and non-phosphorylated regenerated pigments. Basal amounts of arrestin-1 interacted with rhodopsin, 9-cis-retinal-rhodopsin and 13-cis-retinal-rhodopsin under dark and light conditions. Residual arrestin-1 was also recognized by the phosphorylated rhodopsin and phosphorylated 9-cis-retinal-rhodopsin in the dark. However, arrestin-1 was recognized by phosphorylated 13-cis-retinal-rhodopsin in the dark. As expected, all reformed pigments were capable of activating transducin and being phosphorylated by rhodopsin kinase in a lightdependent manner. Additionally, all reconstituted photolyzed and phosphorylated pigments were capable of interacting with arrestin-1. CONCLUSION: In the dark, the rhodopsin analogue containing the 13-cis isomer of retinal appears to fold in a pseudo-active conformation that mimics the active photointermediate of rhodopsin. 展开更多
关键词 rhodopsin rhodopsin ANALOGUES 9-cis-Retinal 11-cis-Retinal 13-cis-Retinal Photointermediates TRANSDUCIN rhodopsin kinase Arrestin-1 Visual process
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Carboxyl terminal of rhodopsin kinase is required for the phosphorylation of photo-activated rhodopsin
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作者 YU QING MING ZHI JIE CHENG +4 位作者 JIAN ZHAO TIAN HUA ZHOU YA LAN WU LAN MA GANG PEI(Shanghai Institute of Cell Biology, Chinese Academy of Science, 320 Yue Yang Road, Shanghai 200031, China)(Department of Neurobiology, Shanghai Medical University,Shanghai 《Cell Research》 SCIE CAS CSCD 1998年第4期303-310,共8页
Human rhodopsin kinase (RK) and a carboxyl terminus-truncated mutant RK lacking the last 59 amino acids (RKC) were expressed in human embryonic kidney 293 cells to investigate the role of the carboxyl terminus of RK i... Human rhodopsin kinase (RK) and a carboxyl terminus-truncated mutant RK lacking the last 59 amino acids (RKC) were expressed in human embryonic kidney 293 cells to investigate the role of the carboxyl terminus of RK in recognition and phosphorylation of rhodopsin. RKC, like the wild-type RK, was detected in both plasma membranes and cytosolic fractions. The Cterminal truncated rhodopsin kinase was unable to phosphorylate photo-activated rhodopsin, but possesses kinase activity similar to the wild-type RK in phosphorylation of small peptide substrate. It suggests that the truncation did not disturb the gross structures of RK catalytic domain. Our results also show that RKC failed to translocate to photo-activated rod out segments. Taken together,our study demonstrate the carboxyl terminus of RK is required for phosphorylation of photo-activated rhodopsin and strongly indicate that carboxyl-terminus of RK may be involved in interaction with photo-activated rhodopsin. 展开更多
关键词 rhodopsin kinase PHOSPHORYLATION fruncation
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Mass genetics study of rhodopsin point mutations in retinitis pigmentosa
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作者 张晓莉 阴正勤 +1 位作者 张雪 府伟灵 《Journal of Medical Colleges of PLA(China)》 CAS 2004年第5期297-301,共5页
Objective: To evaluate the incidence and pattern of rhodopsin (RHO) mutations in Chinese patients with retinitis pigmentosa (RP). Methods: Conformation sensitive gel electrophoresis (CSGE) and direct DNA sequencing we... Objective: To evaluate the incidence and pattern of rhodopsin (RHO) mutations in Chinese patients with retinitis pigmentosa (RP). Methods: Conformation sensitive gel electrophoresis (CSGE) and direct DNA sequencing were applied to detect point mutations that occurred in the five coding exons and splice sites of RHO gene in 98 index patients with RP. Results: Four patients of one ADRP family were found to have a missense mutation at codon 347, Pro347Leu. One late-onset RP patient and her daughter, without clinical expression at present, were discovered to have a novel frameshift mutation at codon 327, Pro327 (1-bp del) . Neither of the two mutations was found in 100 normal controls. Ala299Ser was found in one RP patient. Two control subjects also had Ala299Ser, suggesting its nonpathogenicity and just single nucleotide polymorphism (SNP). Conclusion: Two RP patients had rhodopsin mutations, thus the expected frequency of RHO mutations in RP is about 2.0% (95% confidence interval: 0.3%-4.4%). A highly conserved C-terminal sequence QVS(A) PA was altered due to Pro347Leu and thereby misdirecting rhodopsin to incorrect subcellular location. Loss of all phosphory-lation sites at the C-terminus and a highly conserved sequence QVS(A)PA may occur because of Pro327(1-bp del) . To elucidate the predominant biochemical defects in such mutant, transgenic mice and transfected culture cells carrying Pro327(1-bp del) would be of great value. 展开更多
关键词 retinitis pigmentosa rhodopsin MUTATION conformation sensitive gel electrophoresis SEQUENCING
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Lycium barbarum glycopeptide(wolfberry extract)slows N-methyl-N-nitrosourea-induced degradation of photoreceptors 被引量:1
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作者 Qihang Kong Xiu Han +8 位作者 Haiyang Cheng Jiayu Liu Huijun Zhang Tangrong Dong Jiansu Chen Kwok-Fai So Xuesong Mi Ying Xu Shibo Tang 《Neural Regeneration Research》 SCIE CAS CSCD 2024年第10期2290-2298,共9页
Photoreceptor cell degeneration leads to blindness, for which there is currently no effective treatment. Our previous studies have shown that Lycium barbarum(L. barbarum) polysaccharide(LBP) protects degenerated photo... Photoreceptor cell degeneration leads to blindness, for which there is currently no effective treatment. Our previous studies have shown that Lycium barbarum(L. barbarum) polysaccharide(LBP) protects degenerated photoreceptors in rd1, a transgenic mouse model of retinitis pigmentosa. L. barbarum glycopeptide(Lb GP) is an immunoreactive glycoprotein extracted from LBP. In this study, we investigated the potential protective effect of Lb GP on a chemically induced photoreceptor-degenerative mouse model. Wild-type mice received the following: oral administration of Lb GP as a protective pre-treatment on days 1–7;intraperitoneal administration of 40 mg/kg N-methylN-nitrosourea to induce photoreceptor injury on day 7;and continuation of orally administered Lb GP on days 8–14. Treatment with Lb GP increased photoreceptor survival and improved the structure of photoreceptors, retinal photoresponse, and visual behaviors of mice with photoreceptor degeneration. Lb GP was also found to partially inhibit the activation of microglia in N-methyl-N-nitrosourea-injured retinas and significantly decreased the expression of two pro-inflammatory cytokines. In conclusion, Lb GP effectively slowed the rate of photoreceptor degeneration in N-methyl-N-nitrosourea-injured mice, possibly through an anti-inflammatory mechanism, and has potential as a candidate drug for the clinical treatment of photoreceptor degeneration. 展开更多
关键词 anti-inflammation inherited retinal diseases Lycium barbarum glycopeptide N-METHYL-N-NITROSOUREA OPSIN photoreceptor reactive gliosis retinal degeneration retinitis pigmentosa rhodopsin
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中药跌打膏质量标准提升与安全性研究
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作者 韩杰 金万清 +2 位作者 任国武 谢小中 徐志为 《辽宁中医药大学学报》 CAS 2024年第2期12-18,共7页
目的 建立中药跌打膏质量控制方法,验证中药跌打膏安全性,为临床提供参考。方法 根据配方组成,采用薄层色谱法(TLC)对方中川乌、草乌、大黄、续断、泽兰进行定性鉴别,采用高效液相色谱法(HPLC)定量测定中药跌打膏中大黄素,以用于对中药... 目的 建立中药跌打膏质量控制方法,验证中药跌打膏安全性,为临床提供参考。方法 根据配方组成,采用薄层色谱法(TLC)对方中川乌、草乌、大黄、续断、泽兰进行定性鉴别,采用高效液相色谱法(HPLC)定量测定中药跌打膏中大黄素,以用于对中药跌打膏的质量控制;此外,通过皮肤急性毒性实验、皮肤刺激性实验、皮肤过敏性实验以及豚鼠皮肤组织病理学检查对中药跌打膏的安全性进行评价。结果 该实验中川乌、草乌、大黄、续断、泽兰定性鉴别方法操作简便,分离度好,专属性强。大黄素平均加样回收率为84.917 3%,RSD为1.466 1%。大黄素含量范围为1.099 9%~1.123 8%;精密度、稳定性、重复性试验的RSD分别为0.229 4%、1.835 9%、1.025 0%,均小于3.00%(n=6);安全性实验中,中药跌打膏对小鼠皮肤无刺激性,对小鼠体质量、肝肾功能无影响。一次给药后,14 d观察期间各组小鼠行为活动、精神状态、饮食情况及排便均未出现异常;给药14 d后,取小鼠血液进行血常规检查,后对小鼠进行解剖取血,血常规各项指标及肝肾功能无异常,各脏器未出现肉眼可见病理变化;中药跌打膏干预后的豚鼠皮肤病理检查均未见组织病理学改变。中药跌打膏对豚鼠皮肤无刺激性,中药跌打膏对豚鼠皮肤无明显致敏。结论该实验建立的中药跌打膏中川乌、草乌、大黄、续断、泽兰的TLC鉴别方法和大黄素含量测定方法有良好的精密度、稳定性和重复性,可用于中药跌打膏的质量控制。中药跌打膏对小鼠局部皮肤无毒性,对豚鼠皮肤无刺激性,对豚鼠皮肤无致敏性,说明中药跌打膏外用治疗疾病安全可靠。 展开更多
关键词 中药跌打膏 质量标准 大黄素 皮肤急性毒性 皮肤刺激性 皮肤过敏性
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Heterologous expression and cell membrane localization of dinoflagellate opsins (rhodopsin proteins) in mammalian cells
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作者 Minglei Ma Xinguo Shi Senjie Lin 《Marine Life Science & Technology》 2020年第3期302-308,共7页
Rhodopsins are now found in all domains of life,and are classified into two large groups:type II,found in animals and type I found in microbes including Bacteria,Archaea,and Eukarya.While type II rhodopsin functions i... Rhodopsins are now found in all domains of life,and are classified into two large groups:type II,found in animals and type I found in microbes including Bacteria,Archaea,and Eukarya.While type II rhodopsin functions in many photodependent signaling processes including vision,type 1 among others contains rhodopsins that function as a light-driven proton pump to convert light into ATP as in proteobacteria(named proteorhodopsin).Proteorhodopsin homologs have been documented in dinoflagellates,but their subcellular localizations and functions are still poorly understood.Even though sequence analyses suggest that it is a membrane protein,experimental evidence that dinoflagellate rhodopsins are localized on the plasma membrane or endomembranes is still lacking.As no robust dinoflagellate gene transformation tool was available,we used HEK 293T cells to construct a mammalian expression system for two dinoflagellate rhodopsin genes.The success of expressing these genes in the system shows that this mammalian cell type is suitable for expressing dinoflagellate genes.Immunofluorescence of the expressed protein locates these dinoflagellate rhodopsins on the cell membrane.This result indicates that the protein codons and membrane targeting signal of the dinoflagellate genes are compatible with the mammalian cells,and the proteins'subcellular localization is consistent with proton pump rhodopsins. 展开更多
关键词 Dinoflagellate rhodopsins Proteorhodopsin-Subcellular localization HEK 293T cells
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内质网应激在视网膜色素变性中的作用
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作者 欧晨 谢薇 彭清华 《国际眼科杂志》 CAS 2024年第12期1912-1916,共5页
视网膜色素变性(RP)是以光感受器及色素上皮功能丧失为特征的退行性致盲疾病。内质网应激的激活是细胞的防御调节机制,旨在通过一系列分子信号通路进行自我调节以恢复内质网功能的稳定。视紫红质突变是RP的常见病因,内质网内视紫红质错... 视网膜色素变性(RP)是以光感受器及色素上皮功能丧失为特征的退行性致盲疾病。内质网应激的激活是细胞的防御调节机制,旨在通过一系列分子信号通路进行自我调节以恢复内质网功能的稳定。视紫红质突变是RP的常见病因,内质网内视紫红质错误折叠和滞留,内质网应激诱发感光细胞和视网膜色素上皮细胞凋亡,均可导致RP的发生和发展。文章论述了内质网应激与其在RP发病机制中的作用,并对内质网应激抑制剂、中药和化学药物调控内质网应激在RP治疗中的作用进行总结,以期为内质网应激在RP的临床应用中提供理论依据,为RP的研究、预防和治疗提供新的思路。 展开更多
关键词 内质网应激 视网膜色素变性 视网膜色素上皮细胞 感光细胞 视紫红质
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大黄素联合紫杉醇治疗非小细胞肺癌的作用机制探讨
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作者 王潘红 郑明 蔡云峰 《浙江临床医学》 2024年第3期336-339,共4页
目的 基于网络药理学探讨大黄素联合紫杉醇治疗非小细胞肺癌(NSCLC)的作用机制,并应用实验验证网络药理学结果。方法 通过中药系统药理学分析平台TCMSP以及医药信息查询库药智数据查找大黄素和紫杉醇的相关靶点,人类基因数据库GeneCard... 目的 基于网络药理学探讨大黄素联合紫杉醇治疗非小细胞肺癌(NSCLC)的作用机制,并应用实验验证网络药理学结果。方法 通过中药系统药理学分析平台TCMSP以及医药信息查询库药智数据查找大黄素和紫杉醇的相关靶点,人类基因数据库GeneCards查找NSCLC的相关疾病靶点。应用STRING数据库和Cytoscape构建大黄素联合紫杉醇成分-靶点网络,分析大黄素联合紫杉醇治疗NSCLC的作用靶点、生物学过程以及相关通路,同时利用MTT实验检测大黄素联合紫杉醇对A549细胞增殖的抑制率,并ELISA检测网络药理学得到的核心靶基因水平。结果 大黄素联合紫杉醇与NSCLC的共同靶点基因32个,PPI分析获得前十个靶点蛋白为TP53、CASP3、TNF、EGF、PTGS2、MYC、KDR、TGFB1、MMP9、PPARG,GO分析与KEGG通路分析获得大黄素联合紫杉醇可能作用于NSCLC的150个生物学过程和45条相关通路。MTT结果表明大黄素联合紫杉醇对A549细胞具有明显生长抑制作用(P<0.05),且联合组抑制率明显高于大黄素及紫杉醇单用组(P<0.05)。ELISA结果表明,大黄素与紫杉醇联合组能明显增加A549细胞CASP3含量(P<0.05),降低TNF-α含量(P<0.05),其中联合组效果明显优于大黄素组和紫杉醇组(P<0.05)。结论 大黄素联合紫杉醇能够通过调节细胞增殖与凋亡、调控肿瘤抑制基因表达、炎症反应的相关靶点通路对NSCLC起到治疗作用,大黄素联合紫杉醇有抑制A549细胞增殖的作用,其机制可能与调控CASP3、TNF-α的水平相关。 展开更多
关键词 大黄素 紫杉醇 非小细胞肺癌 GO分析 KEGG分析
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Bidirectional regulation of fragile X mental retardation protein phosphorylation controls rhodopsin hornoeostasis
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作者 Xiao Wang Yawen Mu +1 位作者 Mengshi Sun Junhai Han 《Journal of Molecular Cell Biology》 SCIE CAS CSCD 2017年第2期104-116,共13页
Homoeostatic regulation of the light sensor, rhodopsin, is critical for the maintenance of light sensitivity and survival of photore- ceptors. The major fly rhodopsin, Rhl, undergoes light-induced endocytosis and degr... Homoeostatic regulation of the light sensor, rhodopsin, is critical for the maintenance of light sensitivity and survival of photore- ceptors. The major fly rhodopsin, Rhl, undergoes light-induced endocytosis and degradation, but its protein and mRNA levels remain constant during light/dark cycles. It is not clear how translation of Rhl is regulated. Here, we show that adult photorecep- tors maintain a constant, abundant quantity of ninaE mRNA, which encodes Rhl. We demonstrate that the Fmrl protein associ- ates with ninaE mRNA and represses its translation. Further, light exposure triggers a calcium-dependent dephosphorylation of Fmrl, which relieves suppression of Rhl translation. We demonstrate that Mts, the catalytic subunit of protein phosphatase 2A (PP2A), mediates light-induced Fmrl dephosphorylation in a regulatory B subunit of PP2A (CKa)-dependent manner. Finally, we show that blocking light-induced Rhl translation results in reduced light sensitivity. Our results reveal the molecular mechanism of Rhl homoeostasis and physiological consequence of Rhl dysregulation. 展开更多
关键词 G protein-coupled receptor rhodopsin fragile X mental retardation protein DEPHOSPHORYLATION CALCIUM protein phosphatase 2A
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含好氧不产氧光合基因簇和Xanthorhodopsin-like基因的Sphingomonas sp.MIM37:基因组及光促生长分析 被引量:3
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作者 张星星 刘亚鹏 +3 位作者 袁博 赵吉睿 王瑞刚 冯福应 《微生物学通报》 CAS CSCD 北大核心 2015年第8期1520-1528,共9页
【目的】菌株MIM37为具有两种光能利用途径的光合异养细菌,分析其基因组和光照对生长的影响,为理解光能利用途径、光营养生物多样性以及光合作用的进化和功能等提供线索。【方法】采用平板涂布划线法分离菌株,结合形态观察及16S r RNA... 【目的】菌株MIM37为具有两种光能利用途径的光合异养细菌,分析其基因组和光照对生长的影响,为理解光能利用途径、光营养生物多样性以及光合作用的进化和功能等提供线索。【方法】采用平板涂布划线法分离菌株,结合形态观察及16S r RNA基因和光合基因序列同源性与系统发育分析进行初步分类鉴定;以分光光度法和荧光显微观察法测定光照和黑暗培养下培养液细胞浓度和单细胞体积;构建片段长度为300-500 bp的Illumina PE文库,以Illumina Hiseq2000进行基因组测序,以SOAPdenovo和Gap Closer组装序列,以RAST在线软件注释基因组。【结果】从内蒙古腾格里沙漠天鹅湖表层水中分离获得一株细菌MIM37,经16S r RNA基因、puf M和视紫质基因同源性和系统发育分析均显示其与Sphingomonas属亲缘关系最为密切;相对黑暗培养,光照刺激下的最大细胞浓度和单细胞体积大小分别提高了1.2和5.6倍;基因组注释显示MIM37代谢途径多样,含典型好氧菌的呼吸电子传递链,具有完整的好氧不产氧细菌的光合基因簇及Xanthorhodopsin-like视紫质蛋白基因,合成铁载体,还原重金属,降解微囊藻毒素和多环芳烃类等。【结论】MIM37属于Sphingomonas属,具有两种光能利用途径,光照可明显促进其生长,多样的代谢模式可能使其在自然环境中极具竞争力、分布广泛并具有应用于修复环境污染的潜力。 展开更多
关键词 好氧不产氧光合细菌 光合基因簇 视紫质 16S RRNA pufM 基因组
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大黄素调控P53/P21通路对H_(2)O_(2)诱导损伤HUVEC的保护作用
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作者 宋紫薇 吴铭杰 +3 位作者 李育 赵凤鸣 霍介格 李文婷 《中国老年学杂志》 CAS 北大核心 2023年第20期5029-5032,共4页
目的研究大黄素对过氧化氢(H_(2)O_(2))诱导损伤的血管内皮细胞(HUVEC)保护作用及作用机制。方法MTT法筛选H_(2)O_(2)造模浓度及大黄素给药浓度。取HUVEC细胞,分为正常对照组、H_(2)O_(2)模型组(终浓度100μmol/L H_(2)O_(2))和大黄素4... 目的研究大黄素对过氧化氢(H_(2)O_(2))诱导损伤的血管内皮细胞(HUVEC)保护作用及作用机制。方法MTT法筛选H_(2)O_(2)造模浓度及大黄素给药浓度。取HUVEC细胞,分为正常对照组、H_(2)O_(2)模型组(终浓度100μmol/L H_(2)O_(2))和大黄素4个不同剂量(终浓度15.0、7.5、5.0、2.5μmol/L)组,置于37℃、5%CO_(2)培养箱中培养24 h。电镜和荧光显微镜观察细胞形态和结构,Hoechst法观察细胞凋亡,化学法检测各组细胞中超氧化物歧化酶(SOD)、丙二醛(MDA)、一氧化氮(NO)、一氧化氮合酶(NOS)含量;Western印迹检测各组细胞中P53、半胱氨酸天冬氨酸蛋白酶(caspase)-3和P21蛋白的表达。结果与正常对照组比较,模型组HUVEC细胞增殖活力显著下降;细胞形态与结构改变;SOD、NO、NOS含量显著降低;P53、caspase-3和P21蛋白表达显著提高;经不同剂量大黄素干预后,能明显改善和拮抗H_(2)O_(2)对HUVEC的氧化损伤。结论大黄素对H_(2)O_(2)诱导的HUVEC氧化损伤具有显著保护作用,其作用机制可能是调控P53/P21/caspase-3通路、抑制HUVEC氧化损伤和细胞凋亡。 展开更多
关键词 大黄素 P53/P21通路 过氧化氢(H_(2)O_(2)) 血管内皮细胞(HUVEC) 保护作用
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基于代谢组学探讨犊牛失明原因
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作者 王建东 唐玉林 +4 位作者 郭亚男 高海慧 侯鹏霞 于洋 郭延生 《西南农业学报》 CSCD 北大核心 2023年第10期2281-2291,共11页
【目的】进一步研究犊牛失明的原因,为降低犊牛先天失明的发生率,减少养殖行业经济损失提供理论支持。【方法】选择宁夏地区某牛场出生日期接近的失明犊牛及其母亲、正常犊牛,采集血液收集血浆样本,通过代谢组学分析,对失明犊牛及其母... 【目的】进一步研究犊牛失明的原因,为降低犊牛先天失明的发生率,减少养殖行业经济损失提供理论支持。【方法】选择宁夏地区某牛场出生日期接近的失明犊牛及其母亲、正常犊牛,采集血液收集血浆样本,通过代谢组学分析,对失明犊牛及其母亲、正常犊牛之间差异代谢产物及通路变化进行研究。【结果】将OPLS-DA的VIP值>1和单变量统计分析P<0.05作为显著性差异代谢物的标准,失明犊牛与正常犊牛(VaS.vs.VaL)比较组共筛选出256种差异代谢物,其中正离子模式下144种,负离子模式下112种。失明犊牛与其母亲(VaS.vs.CS)比较组共筛选出177种差异代谢物,其中正离子模式下108种,负离子模式下69种。失明犊牛与其母亲相比,视紫红质含量显著降低,log2FC达-2.87。失明犊牛与其母亲相比,P<0.05差异代谢通路共有30个,矫正后P<0.05的差异代谢通路共有10个,其中胆汁分泌代谢通路分布差异代谢物最多,失明犊牛相较于其母亲有4个代谢物显著上调,9个代谢产物显著下调。失明犊牛与正常犊牛相比,P<0.05差异代谢通路共有12个,矫正后P<0.05的差异代谢通路共有16个,其中胆汁分泌代谢通路分布差异代谢物最多,与正常犊牛相比,失明犊牛有5个代谢物显著上调,4个代谢产物显著下调。【结论】失明犊牛与其母亲、正常犊牛相比胆汁分泌代谢通路均产生显著性差异,研究认为犊牛失明可能是机体自身存在肝脏方面的疾病,影响胆汁的正常分泌,导致正常摄入的脂溶性维生素A不能被吸收利用,进而影响犊牛视力。另外,失明犊牛与其母亲相比,在机体维生素A水平没有显著性差异的条件下,影响光转导级联反应的视紫红质含量显著下调,说明编码视紫红质蛋白的视紫红质基因(RHO)突变,视紫红质蛋白缺乏,可能是导致犊牛失明的另一原因。 展开更多
关键词 犊牛 失明 代谢组学 视紫红质 维生素A缺乏症
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成人骨髓间充质干细胞体外向视网膜细胞的诱导分化 被引量:3
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作者 俞海燕 吴文涛 +1 位作者 王薇 张纯 《中国药理学通报》 CAS CSCD 北大核心 2014年第6期787-791,共5页
目的研究取材于成人骨髓的间充质干细胞在一定诱导条件下向视网膜神经细胞的分化。方法成人骨髓经密度梯度离心得到的细胞,根据其高黏附特性体外培养获得间充质干细胞。利用流式细胞仪分析其细胞表型,在体外诱导使其向视网膜神经细胞分... 目的研究取材于成人骨髓的间充质干细胞在一定诱导条件下向视网膜神经细胞的分化。方法成人骨髓经密度梯度离心得到的细胞,根据其高黏附特性体外培养获得间充质干细胞。利用流式细胞仪分析其细胞表型,在体外诱导使其向视网膜神经细胞分化并用免疫荧光法进行鉴定。结果从骨髓中分离培养的细胞具有成纤维细胞样形态,贴壁生长,表型相对均一,表面标志为CD90、CD44、CD147阳性;而CD34、CD38、CD45、CD14、HLA-DR阴性。体外诱导后可以得到表达nestin(神经干细胞标志物)、GFAP(神经胶质细胞标志物)和Rhodopsin(视网膜光感受器细胞标志物)阳性的细胞。结论从人骨髓中分离培养得到的间充质干细胞具有向视网膜神经细胞分化的潜能。 展开更多
关键词 骨髓 间充质干细胞 视网膜 体外诱导分化 免疫荧光染色 rhodopsin
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温阳益气活血方对遗传性视网膜色素变性小鼠感光细胞凋亡的影响及机制研究 被引量:14
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作者 邓婷婷 窦仁慧 +4 位作者 潘琳 张有花 苑维 邓辉 金明 《中国中西医结合杂志》 CAS CSCD 北大核心 2013年第8期1122-1128,共7页
目的观察中药温阳益气活血方对遗传性视网膜色素变性小鼠视网膜感光细胞凋亡的影响,并探寻其分子机制。方法将RDS(retinal degeneration slow)小鼠随机分为模型组和中药组,并设C57BL/6J小鼠为正常对照组,每组4雌2雄。中药组自雌雄合笼... 目的观察中药温阳益气活血方对遗传性视网膜色素变性小鼠视网膜感光细胞凋亡的影响,并探寻其分子机制。方法将RDS(retinal degeneration slow)小鼠随机分为模型组和中药组,并设C57BL/6J小鼠为正常对照组,每组4雌2雄。中药组自雌雄合笼之日起开始给予温阳益气活血方(10mg/g)灌胃,仔鼠出生后母鼠给予中药水煎液代替日常饮水,仔鼠出生7天开始给予中药水煎剂小剂量灌胃,出生21天按成年鼠剂量灌胃。模型组和正常组同时给予生理盐水灌胃。3组均于仔鼠出生后18、28、48天时采用视网膜电图(electroretinogram,ERG)检测视网膜功能,进行HE染色并计算外核层感光细胞层数,TUNEL法检测感光细胞凋亡率,免疫组织化学染色法计算视紫红质(Rhodopsin)及碱性成纤维细胞生长因子(basicfibro-blast growth factor,bFGF)表达。结果与模型组比较,仔鼠出生后18天时,中药组最大混合反应ERG(Max-ERG)a、b波振幅及bFGF表达明显升高(P<0.05,P<0.01);28、48天时,中药组Max-ERGa、b波振幅明显升高,外核层感光细胞层数明显增加,视网膜感光细胞凋亡率明显降低,Rhodopsin及bFGF表达明显升高,差异均有统计学意义(P<0.05,P<0.01)。结论温阳益气活血方可以有效抑制RDS小鼠感光细胞的凋亡,其机制可能与上调bFGF的表达有关。 展开更多
关键词 温阳益气活血方 视网膜色素变性 感光细胞 凋亡 视紫红质 碱性成纤维细胞生长因子
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视网膜色素变性患者视紫红质基因突变分析 被引量:5
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作者 刘逾 贾晓林 +2 位作者 李进军 卢立志 刘晓玲 《中国全科医学》 CAS CSCD 北大核心 2011年第15期1659-1662,共4页
目的研究中国人视网膜色素变性(RP)患者视紫红质(RHO)基因的突变频率及特征,探讨其在RP发病机制中的作用。方法 运用DNA直接测序法,对55例中国内地汉族RP先证者及55例对照者进行RHO全基因突变检测分析。结果共检出7种碱基变异,其中2种... 目的研究中国人视网膜色素变性(RP)患者视紫红质(RHO)基因的突变频率及特征,探讨其在RP发病机制中的作用。方法 运用DNA直接测序法,对55例中国内地汉族RP先证者及55例对照者进行RHO全基因突变检测分析。结果共检出7种碱基变异,其中2种为非致病错义突变,其余5种为非编码区单核苷酸多态性,RP组和对照组各单核苷酸多态性位点突变频率比较,差异均无统计学意义(P>0.05)。结论 RHO基因在中国华南地区RP患者中的突变率低于国外报道。检出的已报道的单核苷酸多态性位点与RP无显著相关性。 展开更多
关键词 视网膜炎 色素性 视紫质 基因
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牛视紫红质蛋白质中视黄醛的活性位点 被引量:3
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作者 徐四川 邓圣荣 +3 位作者 马丽英 史强 葛茂发 张兴康 《物理化学学报》 SCIE CAS CSCD 北大核心 2009年第7期1290-1296,共7页
视紫红质蛋白是一个跨膜蛋白,视黄醛(RET)在该蛋白中的活性结合位点涉及到视觉过程机理,与一些眼科疾病病理有关.基于牛视紫红质蛋白1U19的蛋白质晶体结构数据,采用密度泛函理论的B3LYP方法计算RET-Lys296残基与视黄醛分子周围半径为0.... 视紫红质蛋白是一个跨膜蛋白,视黄醛(RET)在该蛋白中的活性结合位点涉及到视觉过程机理,与一些眼科疾病病理有关.基于牛视紫红质蛋白1U19的蛋白质晶体结构数据,采用密度泛函理论的B3LYP方法计算RET-Lys296残基与视黄醛分子周围半径为0.6nm的空间范围30个氨基酸残基相互作用和结合能.数值显示1U19蛋白中的残基Glu113、Glu181和Glu122是质子化的RET-Lys296残基的活性结合位点,结合能分别为-333.38、-205.67和-194.56kJ·mol-1.这些氨基酸残基带有一个负电荷,与质子化的RET-Lys296残基发生强烈的离子静电相互作用.另外几个残基Ala292、Cys187、Phe293、Pro291以及Trp265等与质子化RET-Lys296残基也有相互吸引作用.当RET-Lys296残基非质子化,上述相互作用消失,促使视黄醛分子与视蛋白分离.研究发现残基Glu113和Glu181周围各自有一个结晶水分子通过双氢键形式起着稳定作用. 展开更多
关键词 视紫红质 视黄醛 1U19 活性位点 密度泛函理论
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