1.Investigation of metabolic action of Cordyceps sinensis and its cultured mycelia on Escherichia coli by microcalorimetry.
Dan-Lei ZHOU ; Dan YAN ; Bao-Cai LI ; Yan-Shu WU ; Xiao-He XIAO
Acta Pharmaceutica Sinica 2009;44(6):640-644
This study is to investigate the effect of Cordyceps sinensis and its cultured mycelia on growth and metabolism of Escherichia coli, and microcalorimetric method was carried out to evaluate its biological activity. The study will provide the basis for the quality control of Cordyceps sinensis. Experimental result will show the effect of natural Cordyceps sinensis and its cultured mycelia on growth and metabolism of Escherichia coli, with index of P(1max) and effective rate (E) by microcalorimetry, the data of experiment were studied by cluster analysis. The results showed that Cordyceps sinensis and its cultured mycelia not only can promote growth and metabolism of Escherichia coli but also can regulate the balance of intestinal microecology efficiently. When the concentrations of samples > 6.0 mg mL(-1), natural Cordyceps sinensis can promote the growth and metabolism of Escherichia coli efficiently (P < 0.05) compared with the control group, and have better dose-effect relationship with concentration (r > 0.9), its cultured mycelia does not show conspicuous auxoaction (P > 0.05) and have not dose-effect relationship with concentration (r < 0.6); when the concentration of samples < 6.0 mg mL(-1), all samples does not show conspicuous auxoaction (P > 0.05). Natural Cordyceps sinensis and its cultured mycelia can be distinguished by cluster analysis. Microcalorimetry has a good prospect on the quality evaluation of the traditional Chinese medicine.
Biological Products
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pharmacology
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Calorimetry
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methods
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Cordyceps
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Escherichia coli
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drug effects
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growth & development
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Microchemistry
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methods
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Mycelium
2.Advances in the study of synergistic effect of anti-biofilm agents.
Chang-Zhong WANG ; Hui-Juan CHENG
Acta Pharmaceutica Sinica 2012;47(3):339-345
Biofilms are communities of surface-associated bacteria or fungi embedded in a self-produced extracellular polymeric matrix that are notoriously difficult to be eradicated and are sources of many recalcitrant infections. Treatment for biofilm infection with any individual drug is always less effective, while the combinations of different types of drugs are superior to monotherapy concerning the removing of biofilms. This paper focus on research progress in recent years for synergistic effect of drugs in combination against biofilms formed by Pseudomonas aeruginosa, Staphylococcus aureus, Staphylococcus epidermidis, Escherichia coli and Candida albicans.
Anti-Bacterial Agents
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pharmacology
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Antifungal Agents
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pharmacology
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Bacteria
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drug effects
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Biofilms
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drug effects
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growth & development
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Candida albicans
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drug effects
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Escherichia coli
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drug effects
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Pseudomonas aeruginosa
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drug effects
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Staphylococcus aureus
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drug effects
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Staphylococcus epidermidis
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drug effects
3.Electrical impedance method for bacteriological study of drug sensitivity test.
Hongzhi WANG ; Xiaofeng PANG ; Aihua WANG
Journal of Biomedical Engineering 2010;27(4):916-919
In this study, our self-made micro-electrical impedance sensors and experimental apparatus were used to measure the impedance of bacteria-inoculated medium. Then the bacteria in the culture of all values obtained during the period were recorded into the trace impedance curve. Seeing the obvious difference in morphological change, we utilized the differed impedance curves in an attempt to estimate the morphological difference between the drug sensitivity of bacteria. The studies of clinical medicine for achieving rapid drug sensitivity test, automation and intelligentization of drug sensitivity are of practical significance.
Anti-Bacterial Agents
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pharmacology
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Bacteria
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drug effects
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growth & development
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Bacteriological Techniques
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instrumentation
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methods
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Electric Impedance
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Escherichia coli
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drug effects
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growth & development
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Microbial Sensitivity Tests
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methods
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Salmonella
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drug effects
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growth & development
4.Determination of colistin based on biothermal activity detection method.
Yun LUO ; Dan YAN ; Yong-Shen REN ; Shao-Feng ZHANG ; Xue FENG ; Han-Bing LI ; Hui-Ying TANG ; Xiao-He XIAO
Acta Pharmaceutica Sinica 2009;44(10):1136-1139
A biothermal activity detection method has been established to determine the potency of colistin. The biothermal activity fingerprints of E. coli with colistin were determined. There was a good linear relationship (r = 0.993) between logarithm concentration of colistin (lgC) and lag rate of growing time (Deltat%) when the concentrations of colistin ranged from 17.0 to 41.6 u x mL(-1). The average recovery rate was 100.3% (n = 9). Using this method, there was no significant difference between results of colistin potency measurement and those using cup-plate method (P > 0.05). As a result, biothermal activity detection method is sensitive, accurate, rapid, convenient and feasible to determine the potency of colistin. This method can also be applied in real time and online to monitor the process of bacterial growth and could be complementary to the cup-plate method.
Anti-Bacterial Agents
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administration & dosage
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pharmacology
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Calorimetry
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methods
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Colistin
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administration & dosage
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pharmacology
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Dose-Response Relationship, Drug
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Escherichia coli
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drug effects
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growth & development
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Microbial Sensitivity Tests
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methods
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Thermodynamics
5.Microcalorimetric investigation of two cephalosporins on colon bacteria activity.
Fen XU ; Cheng-Gong SONG ; Rui-Hua WU ; Li-Ni YANG ; Li-Xian SUN ; Zong-Bao ZHAO ; Zhi-Heng ZHANG ; Zhong CAO ; Ling ZHANG
Acta Pharmaceutica Sinica 2009;44(10):1127-1130
The effects of cephradinum and ceftazidime on the metabolism of Escherichia coli (E. coli) DH5alpha was determined by microcalorimetry. The microbial activity was recorded as power-time curves through an ampoule method with a TAM Air Isothermal Microcalorimeter at 37 degrees C. The parameters such as the growth rate constant (k), inhibitory ratio (I), the maximum power output (Pm) and the time (tm) corresponding to the maximum power output were calculated. The results show that the ceftazidime has a better inhibitory effect on E. coli DH5alpha than cephradinum.
Anti-Bacterial Agents
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administration & dosage
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pharmacology
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Calorimetry
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methods
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Ceftazidime
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administration & dosage
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pharmacology
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Cephradine
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administration & dosage
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pharmacology
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Escherichia coli
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drug effects
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growth & development
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metabolism
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Microbial Sensitivity Tests
6.An exploration of the preventive effects on lanthanum chloride on enteral bacterial translocation in scalded rats.
Qiang LIU ; Yongmo ZHANG ; Guohui LI ; Yong CAO ; Qinghong HU ; Xieqing WU ; Xiaochun ZHONG ; Wen WANG ; Nianyun WANG
Chinese Journal of Burns 2002;18(2):81-83
OBJECTIVETo explore the preventive effect of lanthanum chloride on enteral bacterial translocation in scalded rats.
METHODSNinety Sprague-Dawley (SD) rats were employed in the study and randomly divided into three groups, i.e. normal control (A), burn control (B) and treatment (C) groups. Plasmid PUC19 labelled by JM109 was transfected to Escherichia coli (E. coli), so that restriction endonuclease finger - print image spectrum analysis could be applied to the tracing and quantification of the translocation of E. coli from intestine to mesenteric lymph nodes (MLNs) and blood. The intestinal tissue contents of endotoxin (ET), nitric oxide (NO), nitric oxide synthase (NOS), malondialdehyde (MDA) and superoxide dismutase (SOD) were determined.
RESULTSIt was identified that the bacteria in MLNs and blood exhibited the same gene map with those from gastric gavage in B and C groups. But the bacterial quantity in MLNs in C group on 3 postburn day (PBD) was much lower than that in B group (P < 0.05). The intestinal MDA content in C group on 1 and 3 PBDs was obviously higher than that in B group (P < 0.05).
CONCLUSIONBacteria (E. coli) could be translocated from gut to MLNs and blood, which could be evidently alleviated by lanthanum chloride by means of its bactericidal property, inhibition of NOS activity, so that NO production decreased, and its ability to increase SOD activity leading to less production of MDA.
Animals ; Burns ; drug therapy ; microbiology ; Endotoxins ; blood ; metabolism ; Escherichia coli ; drug effects ; growth & development ; metabolism ; Escherichia coli Infections ; blood ; microbiology ; prevention & control ; Female ; Intestines ; drug effects ; metabolism ; microbiology ; Lanthanum ; pharmacology ; Lymph Nodes ; drug effects ; microbiology ; Male ; Malondialdehyde ; blood ; metabolism ; Mesentery ; drug effects ; microbiology ; Nitric Oxide ; blood ; metabolism ; Nitric Oxide Synthase ; blood ; metabolism ; Rats ; Rats, Sprague-Dawley ; Superoxide Dismutase ; blood ; metabolism
7.Biocompatibility of SA/CS-CaCl2/PMCG Microcapsule in cell culture.
Li-Yang ZHANG ; Yi-Xin GUAN ; Shan-Jing YAO
Chinese Journal of Biotechnology 2002;18(6):709-712
A novel multi-components microcapsule--SA/CS-CaCl2/PMCG system was introduced. The effects of PMCG and SA/CS-CaCl2/PMCG microcapsules on the growth of free E. coli and Saccharomyces cerevisiae were studied respectively. In addition, the growth of immobilized E. coli and Saccharomyces cerevisiae were also investigated. The results showed that: Just like other synthetic polycations, PMCG above certain concentration (0.5%) strongly inhibited the growth of free E. coli and Saccharomyces cerevisiae, but SA/CS-CaCl2/PMCG microcapsules almost had no effects on their growth and on the consumption of glucose concentration by Saccharomyces cerevisiae. What's more, immobilized E. coli and Saccharomyces cerevisiae grew almost as normally as free cultivation. As a whole, SA/CS-CaCl2/PMCG microcapsules had good biocompatiability and can be used as a new immobilization system.
Alginates
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toxicity
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Biocompatible Materials
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toxicity
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Calcium Chloride
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toxicity
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Cellulose
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analogs & derivatives
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toxicity
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Escherichia coli
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drug effects
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growth & development
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Glucuronic Acid
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Hexuronic Acids
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Polymers
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toxicity
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Saccharomyces cerevisiae
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drug effects
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growth & development
8.Refolding and purification of recombinant human VEGF-121 expressed as inclusion bodies in Escherichia coli.
Zhi-ming HU ; Li MA ; Ming-qian ZHOU ; Ji-min GAO ; Xiao-ning WANG
Journal of Southern Medical University 2006;26(8):1083-1086
Vascular endothelial growth factor 121 (VEGF(121)) was expressed as inclusion bodies by recombinant Escherichia coli. High concentrations of both biomass (46 g dry cell/L) and VEGF(121) inclusion bodies (4.5 g/L) were obtained by applying a high-cell-density culture. After the inclusion bodies were washed and dissolved, VEGF(121) was refolded at 0.2 mg/ml by ultrafiltration in refolding buffer with a yield of 81%. Renatured VEGF(121) was purified by anion chromatography and Sephacry S-100 chromatography with purity higher than 95% and final purification yield of 31%. The purified VEGF(121) could stimulate the proliferation of human umbilical vein endothelial cells as demonstrated by a biological activity assay.
Cell Line
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Cell Proliferation
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drug effects
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Dose-Response Relationship, Drug
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Endothelial Cells
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cytology
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drug effects
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Escherichia coli
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genetics
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metabolism
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Humans
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Inclusion Bodies
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metabolism
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Protein Folding
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Recombinant Proteins
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biosynthesis
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chemistry
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isolation & purification
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Vascular Endothelial Growth Factor A
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biosynthesis
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genetics
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pharmacology
9.Evaluation methods for quality volatility about yiqi fumai freeze-dried powder used for injection based on bio-thermodynamics exosyndrome.
Yan YAN ; Dan YAN ; Ping ZHANG ; Zhengliang YE ; Dazheng ZHOU ; Xiaohe XIAO
China Journal of Chinese Materia Medica 2012;37(1):41-45
Yiqi Fumai freeze-dried powder for injection was used as a model drug to establish an evaluation method mainly based on bio-thermodynamics profile detection. Fischer function was used to analyze the chemical and biological data In general, chemical chromatogram can distinguish the expired sample and thermal spectrum of biological activity can distinguish special samples exactly. Thus, we established the evaluation method regarding the quality volatility of Yiqi Fumai freeze-dried powder for injection. The method can be used as a useful supplement in quality control as, and it could provide some technical information for quality control of other varieties of traditional Chinese medicine for injection.
Biological Assay
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methods
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Chromatography, High Pressure Liquid
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methods
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Drug Therapy
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Drugs, Chinese Herbal
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chemistry
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pharmacology
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standards
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Escherichia coli
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chemistry
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drug effects
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growth & development
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Humans
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Kinetics
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Powders
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chemistry
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pharmacology
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standards
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Quality Control
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Thermodynamics
10.Protoplast transformation of Mortierella isabellina with hygromycin B resistance plasmid PD4.
Xue-Wei ZHANG ; Xiao-Mei WANG ; Ming-Chun LI ; Dong-Sheng WEI ; Xue CHEN ; Lai-Jun XING
Chinese Journal of Biotechnology 2007;23(3):462-466
A strain Mortierella isabellina M6-22-4, which was sensitive to hygromycin B, was selected by treating parental spores with N-methyl-N' -Nitro-N-nitrosoguanidine (MNNG). Protoplasts of the strain Mortierella isabellina M6-22-4 were transformed successfully to hygromycin B resistance using the PD4 plasmid, which contains the Escherichia coli hph gene under the control of Mortierella alpina his H4.1 promoter. The PD4 plasmid was introduced by PEG/CaCl2 treatment. Transformation frequencies of 1.6 - 2.8 transformants/microg of DNA were achieved. Then they were successively incubated to non-selected PDA plates for 10 generations. About 31.6% transformants only from digested plasmid were mitotically stable and showed different hygromycin B resistance when they were incubated back to selection plates. The results of PCR and Southern analysis in three transformants indicated that the plasmid PD4 had been integrated into the fungal genome with 1 - 2 copies. This is the first report of Mortierella isabellina transformation system and supplies an important tool for further research into genetic manipulation of this filamentous fungus.
Anti-Bacterial Agents
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pharmacology
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Blotting, Southern
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Drug Resistance, Microbial
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genetics
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Escherichia coli Proteins
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genetics
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Genome, Fungal
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genetics
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Hygromycin B
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pharmacology
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Mortierella
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drug effects
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genetics
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growth & development
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Plasmids
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genetics
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Polymerase Chain Reaction
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Protoplasts
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metabolism
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Transformation, Genetic