期刊文献+
共找到13篇文章
< 1 >
每页显示 20 50 100
一种新的测定血管壁通透性的方法
1
作者 林海 龚肖崎 +1 位作者 钟纪根 陈骏 《微循环学杂志》 1995年第3期28-29,共2页
给SD大鼠静脉注射荧光标记白蛋白,通过检测其肺、肾组织匀浆中荧光标记白蛋白的含量,定量分析其血管壁通透性变化。该方法与伊文氏蓝方法相比,能更准确反映血管壁对大分子物质的通透性的变化,又避免了使用核素标记白蛋白时放射性... 给SD大鼠静脉注射荧光标记白蛋白,通过检测其肺、肾组织匀浆中荧光标记白蛋白的含量,定量分析其血管壁通透性变化。该方法与伊文氏蓝方法相比,能更准确反映血管壁对大分子物质的通透性的变化,又避免了使用核素标记白蛋白时放射性的污染,为进一步研究血管壁通透性的变化提供了一种更准确而又方便的新方法。本实验还测定了烫伤12h后大鼠肺、肾血管壁通透性的变化。 展开更多
关键词 血管壁通透性 测定 荧光白蛋白
下载PDF
Interaction Between Gatifloxacin and Bovine Serum Albumin 被引量:7
2
作者 严拯宇 邵秀芬 +1 位作者 严琳 胡育筑 《Journal of Chinese Pharmaceutical Sciences》 CAS 2005年第1期33-37,共5页
Aim To study the reaction mechanism between gatifloxacin and bovine serumalbumin (BSA) at different pHs. Methods Fluorescence spectra and UV absorbance spectra were used.Results The binding constants were determined f... Aim To study the reaction mechanism between gatifloxacin and bovine serumalbumin (BSA) at different pHs. Methods Fluorescence spectra and UV absorbance spectra were used.Results The binding constants were determined from a double reciprocal Lineweaver-Burk curves atdifferent pHs. The binding distance r under normal physiological condition was obtained according toFoster theory of non-radiative energy transfer. The binding force between gatifloxacin and BSA wasinferred by thermody-namical coordination. Conclusion The interaction between gatifloxacin and BSAseems to be strong and the main binding force is electrostatic force. 展开更多
关键词 fluorescence quenching bovine serum albumin GATIFLOXACIN
下载PDF
Construction and expression of GFP conjugated MIM-I-BAR
3
作者 曹萌 常维维 +3 位作者 许阳 方琳静 刘袁 顾宁 《Journal of Southeast University(English Edition)》 EI CAS 2015年第3期353-357,共5页
To achieve a visible inverse Bin-amphiphysin-Rvs (I-BAR)domain recombinant of missing in metastasis (MIM) protein,the green fluorescent protein (GFP)encoding gene was cloned at the terminal of MIM-I-BAR as a pro... To achieve a visible inverse Bin-amphiphysin-Rvs (I-BAR)domain recombinant of missing in metastasis (MIM) protein,the green fluorescent protein (GFP)encoding gene was cloned at the terminal of MIM-I-BAR as a probe.The DNA was successfully constructed on a 6xHis-tagged prokaryotic expression plasmid.The non-GFP labeled MIM-I-BAR encoding plasmid was also constructed as a control. Being successfully transformed into BL21 (DE3 )cells,the GFP-conjugated MIM-I-BAR (MIM-I-BAR-GFP ) exhibits strong visible fluorescence,and the expression product can be easily detected by visual inspection, a fluorescence microscope, Western blot or ultraviolet and visible spectrophotometer. Moreover, examination of expression efficiency under various culture conditions revealed that the MIM-I-BAR-GFP gene has a high protein yield at 10 ℃,but not at the culture temperature of 37 ℃.This property is much different from that of the non-fluorescent MIM-I-BAR gene. This optimal expression condition is also proved to be feasible for protein production in midi-scale. The fluorescent recombinant MIM-I-BAR-GFP protein can serve as a useful tool in scientific research, biomedical application and pharmaceutical development. 展开更多
关键词 inverse Bin-amphiphysin-Rvs missing in metastasis inverse Bin-amphiphysin-Rvs green fluorescent protein plasmid EXPRESSION purifica-tion
下载PDF
Intrahepatic transplantation of hepatic oval cells for fulminant hepatic failure in rats 被引量:7
4
作者 Chen-Xuan Wu,Qi Zou,Zheng-Yan Zhu,Ying-Tang Gao,Yi-Jun Wang,Department of Hepatobiliary,The Third Center of Affiliated Hospital of Tianjin Medical University Key Laboratory of Artificial Cells of Tianjin,Tianjin 300170,China Author contributions:Wang YJ,Wu CH and Zou Q designed the research +2 位作者 Zou Q,Zhu ZY,Gao YT performed the research Zou Q analyzed the data Wang YJ and Wu CX wrote the paper.Supported by Tianjin Science Committee,Grant No.05SYSYJC02600 and Tianjin Health Bureau,Grant No.05KYR01 《World Journal of Gastroenterology》 SCIE CAS CSCD 2009年第12期1506-1511,共6页
AIM: To evaluate the effect of intrahepatic transplantation of hepatic oval cells (HOC) on fulminant hepatic failure (FHF) in rats.METHODS: HOC obtained from rats were labeled with green fluocescent protein (GF... AIM: To evaluate the effect of intrahepatic transplantation of hepatic oval cells (HOC) on fulminant hepatic failure (FHF) in rats.METHODS: HOC obtained from rats were labeled with green fluocescent protein (GFP) or 5, 6- carboxyfluorescein diacetate succinmidyl ester (CFDASE). Cell fluorescence was observed under fluorescent microscope at 6, 24, 48 and 72 h after labeling. CFDA- SE labeled HOC (5 × 10^6 cells each rat) were injected into livers of rats with FHF induced by D-galactosamine. Serum albumin (ALB), alanine aminotransferase (ALT), aspartate aminotransferase (AST) and total bilirubin (TBil) levels were measured at different time points. Liver function of rats was examined on days 3, 7, 14 and 21 after HOC transplantation.RESULTS: The positive rate of GFP and CFDA-SE labeled HOC was 10% and 90%, respectively, with no significant change in cell viabilities. The survival rate was higher in HOC transplantation group than in control group, especially 48 (9/15 vs 6/15) and 72 h (9/15 vs 4/15) after HOC transplantation. The serum ALT, AST and TBil levels were decreased while the serum AIb level was increased after HOC transplantation. Fluorescence became faded and diffused in liver tissues, suggesting that proliferation and differentiation occur in transplanted HOC.CONCLUSION: CFDA-SE is superior to GFP in labeling HOC, although fluorescence intensity is decreased progressively with cell division. HOC transplantation can improve the liver function and increase the survival rate of recipients. 展开更多
关键词 LIVER Stem cells Hepatic oval cells Fluorescence labeling TRANSPLANTATION Fulminanthepatic failure
下载PDF
Preparation and Charaterization of Self-assembled Nanoparticles Based on Linolenic-acid Modified Chitosan 被引量:6
5
作者 LIU Chenguang Desai Kashappa Goud H. +1 位作者 CHEN Xiguang Park Hyun-Jin 《Journal of Ocean University of China》 SCIE CAS 2005年第3期234-239,共6页
Chitosan was modified by conjugating coupling with linolenic acid through the 1-ethyl-3-(3-dimethylami- nopropyyl) carbodiimide (EDC)-mediated reaction. The degree of substitution 1.8% ( i.e. 1.8 linolenic acid g... Chitosan was modified by conjugating coupling with linolenic acid through the 1-ethyl-3-(3-dimethylami- nopropyyl) carbodiimide (EDC)-mediated reaction. The degree of substitution 1.8% ( i.e. 1.8 linolenic acid group per 100 anhydroglucose units) was measured by ^1H NMR. The critical aggregation concentration (CAC) of the self-aggregate of hydrophobically modified chitosan was determined by measuring the fluorescence intensity of the pyrene as a fluorescent probe. The CAC value in phosphate-buffered saline (PBS) solution (pH 7.4) was 5 × 10^-2 mg mL^-1. The average particle size of selfaggregates of hydrophobically modified chitosan in PBS solution (pH7.4) was 210.8 nm with a unimodal size distribution ranging from 100 to 500 nm. Transmission electron microscopy (TEM) study showed that the formation of near spherical shape nanoparticles has enough structural integrity. The loading ability of hydrophibically modified chitosan (LA-chitosan) was investigated by using bovine serum albumin (BSA) as the model. The loading capacity of self-aggregated nanoparticles increases ( 19.85 % ± 0.04 % to 37.57 % ± 0.25 % ) with the concentration of BSA (0.1-0.5 mg mL^-1 ). 展开更多
关键词 CHITOSAN linolenic acid NANOPARTICLES self-aggregates BSA
下载PDF
Binding interactions of pefloxacin mesylate with bovine lactoferrin and human serum albumin 被引量:2
6
作者 FAN Ji-cai CHEN Xiang WANG Yun FAN Cheng-ping SHANG Zhi-cai 《Journal of Zhejiang University-Science B(Biomedicine & Biotechnology)》 SCIE CAS CSCD 2006年第6期452-458,共7页
The binding of pefloxacin mesylate (PFLX) to bovine lactoferrin (BLf) and human serum albumin (HSA) in dilute aqueous solution was studied using fluorescence spectra and absorbance spectra. The binding constant ... The binding of pefloxacin mesylate (PFLX) to bovine lactoferrin (BLf) and human serum albumin (HSA) in dilute aqueous solution was studied using fluorescence spectra and absorbance spectra. The binding constant K and the binding sites n were obtained by fluorescence quenching method. The binding distance r and energy-transfer efficiency E between pefloxacin mesylate and bovine lactoferrin as well as human serum albumin were also obtained according to the mechanism of Forster-type dipole-dipole nonradiative energy-transfer. The effects of pefloxacin mesylate on the conformations of bovine lactoferrin and human serum albumin were also analyzed using synchronous fluorescence spectroscopy. 展开更多
关键词 Pefloxacin mesylate (PFLX) Bovine lactoferrin (BLf) Human serum albumin (HSA) Fluorescence spectra Energy-transfer efficiency
下载PDF
Effect of Yiguanjian decoction on cell differentiation and proliferation in CCl_4-treated mice 被引量:4
7
作者 Xiao-Ling Wang Dong-Wei Jia +6 位作者 Hui-Yang Liu Xiao-Feng Yan Ting-Jie Ye Xu-Dong Hu Bo-Qin Li Yong-Liang Chen Ping Liu 《World Journal of Gastroenterology》 SCIE CAS CSCD 2012年第25期3235-3249,共15页
AIM: To investigate the cellular mechanisms of action of Yiguanjian (YGJ) decoction in treatment of chronic hepatic injury. METHODS: One group of mice was irradiated, and received enhanced green fluorescent prote... AIM: To investigate the cellular mechanisms of action of Yiguanjian (YGJ) decoction in treatment of chronic hepatic injury. METHODS: One group of mice was irradiated, and received enhanced green fluorescent protein (EGFP)- positive bone marrow transplants followed by 13 wk of CCh injection and 6 wk of oral YGJ administration. A second group of Institute for Cancer Research mice was treated with 13 wk of CCI4 injection and 6 wk of oral YGJadministration. Liver function, histological changes in the liver, and Hyp content were analyzed. The expres- sion of m-smooth muscle actin (α-SMA), F4/80, albumin (AIb), EGFP, mitogen-activated protein kinase-2 (PKM2), Ki-67, fetoprotein (AFP), monocyte chemotaxis pro- tein-1 and CC chemokine receptor 2 were assayed. RESULTS: As hepatic damage progressed, EGFP-po- sitive marrow cells migrated into the liver and were mainly distributed along the fibrous septa. They showed a conspicuous coexpression of EGFP with ^-SMA and F4/80 but no coexpression with AIb. Moreover, the expression of PKM2, AFP and Ki-67 was enhanced dy- namically and steadily over the course of liver injury. YGJ abrogated the increases in the number of bone marrow-derived fibrogenic cells in the liver, inhibited expression of both progenitor and mature hepatocyte markers, and reduced fibrogenesis. CONCLUSION: YGJ decoction improves liver fibrosis by inhibiting the migration of bone marrow cells into the liver as well as inhibiting their differentiation and suppressing the proliferation of both progenitors and hepatocytes in the injured liver. 展开更多
关键词 Yiguanjian decoction Bone marrow trans-plantation Hepatic progenitors HEPATOCYTES Hepaticinjury
下载PDF
Expression and characterization of Mac-1-FP fusion protein in CHO cells
8
作者 刁飞 严鸣 +3 位作者 朱晓燕 杨勇骥 刘辉 徐仁宝 《Journal of Medical Colleges of PLA(China)》 CAS 2004年第6期321-324,共4页
Objective: To construct mammalian cell expression vectors for Mac-1 with CFP and YFP and apply FRET to study the dimerization and function of CD11 b( Mac-1 α subunit) and CD18(Mac-1 β subunit). Methods: The mammalia... Objective: To construct mammalian cell expression vectors for Mac-1 with CFP and YFP and apply FRET to study the dimerization and function of CD11 b( Mac-1 α subunit) and CD18(Mac-1 β subunit). Methods: The mammalian cell expression vector for CD11b fused with CFP at the carboxyl terminal was constructed to create recombinant plasmid of pCD11b-CFP. Then pCD11b-CFP was co-transfected with pYFP-CD18 into CHO cell, a fibroblast like cell line, as a target cell within which there are some signal pathways involved in inflammatory stimulation but without endogenous Mac-1. Then CHO cells stably expressing both CD11b-CFP and YFP-CD18 fusion proteins were selected by Western blot and laser scanning confocal microscope. Results: The cyan and yellow fluorescence in co-transfected positive CHO cells were observed under a fluorescence microscope. CHO-Mac-1-FP cells stably expressing both CD11b-CFP and YFP-CD18 fusion proteins were obtained as demonstrated by Western blot successfully. The adhesive activity of CHO-Mac-1-FP cells with CHO-1CAM-1 cells was increased markedly by treatment with PMA, suggesting the translocation of GD11b-CFP and YFP-CD18 to the plasma membrane in CHO-Mac-1-FP cells and dimerization of CD11b-CFP and YFP-CD18 just as the function of the wild type Mac-1. Conclusion: CHO-Mac-1-FP cells with adhesive activity are established successfully, thus CHO-Mac-1-FP cells may be useful for the study of Mac-1 by FRET and for other purposes. 展开更多
关键词 MAC-1 cyan fluorescent protein yellow fluorescent protein fusion protein
下载PDF
Fluorescent Proteins as a Visible Molecular Signal for Rapid Quantification of Bioprocesses: Potential and Challenges 被引量:3
9
作者 张翀 邢新会 《Chinese Journal of Chemical Engineering》 SCIE EI CAS CSCD 2010年第5期863-869,共7页
Green fluorescent protein (GFP) and its variants /homolog proteins are generally called as GFP-like fluorescent proteins (FPs), which are widely used as visible molecular tools for monitoring a wide range of biologica... Green fluorescent protein (GFP) and its variants /homolog proteins are generally called as GFP-like fluorescent proteins (FPs), which are widely used as visible molecular tools for monitoring a wide range of biological processes due to their capability of simple, accurate and real time quantification. The FPs-based molecular and visible quantification tools are giving more impact on bioprocess engineering, enabling the biomolecule-level dynamic information to be linked with the process-level events. In this review, different applications of FPs in biological engineering with emphasis on rapid molecular bioprocess quantification, such as quantification of the transcription efficiency, the protein production, the protein folding efficiency, the cell concentration, the intracellular microenvironments and so on, would be first introduced. The challenges of using FPs with respect to actual bioprocess applications for the precise quantification including the interaction of FPs and the fused partner proteins, the maturation of FPs, the inner filter effect and sensing technology were then discussed. Finally, the future development for the FPs used in molecular bioprocess quantification would be proposed. 展开更多
关键词 green fluorescent protein fluorescent proteins bioprocess engineering quantification MARKER
下载PDF
Surface Display of Domain Ⅲ of Japanese Encephalitis Virus E Protein on Salmonella Typhimurium by Using an Ice Nucleation Protein 被引量:2
10
作者 Jian-lin Dou Tao Jing +1 位作者 Jingojing Fan Zhi-ming Yuan 《Virologica Sinica》 SCIE CAS CSCD 2011年第6期409-417,共9页
A bacterial cell surface display technique based on an ice nucleation protein has been employed for the development of live vaccine against viral infection. Due to its ubiquitous ability to invade host cells, Salmonel... A bacterial cell surface display technique based on an ice nucleation protein has been employed for the development of live vaccine against viral infection. Due to its ubiquitous ability to invade host cells, Salmonella typhimurium might be a good candidate for displaying viral antigens. We demonstrated the surface display of domain III of Japanese encephalitis virus E protein and the enhanced green fluorescent protein on S. typhimurium BRD509 using the ice nucleation protein. The effects of the motif in the ice nucleation protein on the effective display of integral protein were also investigated. The results showed that display motifs in the protein can target integral foreign protein on the surface of S. typhimurium BRD509. Moreover, recombinant strains with surface displayed viral proteins retained their invasiveness, suggesting that the recombinant S. typhimurium can be used as live vaccine vector for eliciting complete immunogenicity. The data may yield better understanding of the mechanism by which ice nucleation protein displays foreign proteins in the Salmonella strain. 展开更多
关键词 Cell surface display Ice nucleation protein Salmonella typhimurium Japanese encephalitis virus
下载PDF
A bacterial artificial chromosome transgenic mouse model for visualization of neurite growth 被引量:1
11
作者 TAO Tao CHEN Chen +2 位作者 SUN Jie PENG YaJing ZHU MinSheng 《Science China(Life Sciences)》 SCIE CAS CSCD 2015年第4期373-378,共6页
Class Ⅲ β-tubulin (Tubb3) is a component of the microtubules in neurons and contributes to microtubule dynamics that are required for axon outgrowth and guidance during neuronal development. We here report a novel... Class Ⅲ β-tubulin (Tubb3) is a component of the microtubules in neurons and contributes to microtubule dynamics that are required for axon outgrowth and guidance during neuronal development. We here report a novel bacterial artificial chromosome (BAC) transgenic mouse line that expresses Class Ⅲ β-tubulin fused to mCherry, an improved monomeric red fluorescent protein, for the visualization of microtubules during neuronal development. A BAC containing Tubb3 gene was modified by insertion of mCherry complementary DNA downstream of Tubb3 coding sequence via homologous recombination, mCherry fusion protein was expressed in the nervous system and testis of the transgenic animal, and the fluorescent signal was observed in the neurons that located in the olfactory bulb, cerebral cortex, hippocampal formation, cerebellum, as well as the retina. Besides, Tubb3-mCherry fusion protein mainly distributed in neurites and colocalized with endogenous Class Ⅲ β-tubulin The fusion protein labels Purkinje cell dendrites during cerebellar circuit formation. Therefore, this transgenic line might be a novel tool for scientific community to study neuronal development both in vitro and in vivo. 展开更多
关键词 Tubb3 MCHERRY BAC transgenic mouse neuronal development Purkinje cells
原文传递
Enhancement of fluorescence of terbium and transferrin-bound diterbium by HEPES
12
作者 杜萍 袁兰 +2 位作者 吴后男 徐克宁 杨晓改 《Journal of Chinese Pharmaceutical Sciences》 CAS 2009年第3期218-224,共7页
Terbium (Tb) has been extensively used as a fluorescence probe for the identification of calcium-binding sites in proteins and for fluorometric analysis of organic ligands. In the current study, we reported that HEP... Terbium (Tb) has been extensively used as a fluorescence probe for the identification of calcium-binding sites in proteins and for fluorometric analysis of organic ligands. In the current study, we reported that HEPES, a commonly used pH buffer reagent, significantly enhanced the characteristic emission of Tb at 585 nm. The maximum emission of Tb at 490 nm and 549 um were also enhanced by HEPES to a less extent. Thus, cautions should be taken when quantitative analysis is performed based on the fluorescence emission of Tb at 549 nm, since the emission may vary due to the buffer reagents. Additionally, the fluorescence intensity at 585 um was proportional to the concentration of both HEPES and terbium ions, which might be utilized to develop new fluorometric analytical methods. 展开更多
关键词 Tb^3+ HEPES FLUORESCENCE Tb2Tf ApoTf
原文传递
Interaction of epicatechin with bovine serum albumin using fluorescence quenching combined with chemometrics 被引量:2
13
作者 ZHAI Min WU HaiLong +3 位作者 ZHANG ShuRong ZHANG XiHua SUN YanMei YU RuQin 《Science China Chemistry》 SCIE EI CAS 2014年第5期748-754,共7页
The interaction between BSA and epicatechin was studied using fluorescence quenching titrations combined with trilinear decomposition method and excitation-emission matrix(EEM)fluorescence.The resolved spectra were hi... The interaction between BSA and epicatechin was studied using fluorescence quenching titrations combined with trilinear decomposition method and excitation-emission matrix(EEM)fluorescence.The resolved spectra were highly similar with the actual ones which indicated that the resolved results were reliable.The relevant parameters of the binding process were obtained by quantifying each substance in the complicated mixtures in situ.The quenching was static quenching,epicatechin had a weak interaction with BSA and the binding site was one.The total concentration and the free concentration of quenchers had different effect on the system.The results demonstrated that the method exploited in this article is a useful tool to investigate complicated interactions,avoiding complicated pretreatment and simplify experimental procedure. 展开更多
关键词 EPICATECHIN bovine serum albumin three-dimensional fluorescence quenching trilinear decomposition method in situinterpretation of binding parameters
原文传递
上一页 1 下一页 到第
使用帮助 返回顶部