C8-oxo-HSl对P.aeruginosa在污水处理中生长特性影响

通过24孔板序批实验对群体效应(QS)信号分子C_8-oxo-HSL对铜绿假单胞菌(P.aeruginosa)在污水处理过程中生长特性影响作用进行分析探讨.研究发现C_8-oxo-HSL有效刺激P.aeruginosa大量生长,其对应的阙值浓度为10^(-10)g/L C_8-oxo-HSL.同时推知具有Lux I/R群体效应系统的革兰氏阴性菌可在较低的信号分子浓度作用下大量增殖.C_8-oxo-HSL还可有效刺激P.aeruginosa分泌大量蛋白质至紧密型胞外聚合物(TB-EPS)中,其对应的阙值浓度为10^(-7)g/LC_8-oxo-HSL.但C_8-oxo-HSL对P.aeruginosa的TB-EPS中多糖没有明显影响作用.C_8-oxo-HSL通过促使P.aeruginosa的增殖和团聚从而增强菌胶团稳定性.此外C_8-oxo-HSL可促进P.aeruginosa生物膜形成.但由于P.aeruginosa生物膜的形成同时和细菌菌量与胞外聚合物浓度直接相关.所以P.aeruginosa生物膜快速生长的C_8-oxo-HSL阙值浓度相对较高(约10^(-8)g/L).

The effect of Some Boron Derivatives on Kanamycin Resistance and Survival of E.coli and P.aeruginosa in Lake Water

Objective To study MIC value of 7 boron derivatives namely [Boric acid （H3BO3）, Anhydrous Borax （Na2B407）, Sodium Borate （NaBO2）, Diammonium Tetraborate （NH4）2B4O7, Sodium Perborate （NaBO3）, Boron Trioxide （B203）, Potassium Tetraborate （K2B407）] on E. coil and P. aeruginosa and their effects on survival of bacteria in lake water and resistance against kanamycin antibiotic. Methods MIC values of Boron derivatives and antibiotic were studied by broth microdilution method. The effect of boron derivatives on survival of bacteria in lake water were also determined with plate count. Results Sodium perborate was determined as the substances. Effectiveness increased as temperature most effective substance among the studied increased. E. coil was more affected from P. aeruginosa in 8 mg/mL sodium perborate concentration in lake water. Moreover, it was determined that MIC value of kanamycin antibiotic decreased 200 times by especially treating P. aeruginosa with sodium perborate in lake water. However, it can be stated that this change in resistance did not arise from microorganisms. Conclusion Sodium perborate solution can be used supportedly in kanamycin antibiotic applications for P. aeruginosa. Future studies are necessary to explore the relation between sodium perborate and kanamycin which is effective on P. aeruginosa in lake water.

Analysis of Drug Resistance Spectra and Conjugative Plasmid Carrying Rates of P.aeruginosa and Acinetobacter

Antimicrobial susceptibility test was performed on 57 clinical isolates of P. aeruginosa and 36 clinical isolates of Acinetobacter with 11 antimicrobial agents including getamicin, amikacin, ciprofloxacin, ofloxacin, fleroxacin, piperacillin, cefotaxime, cefoperazone/sulbactam, ceftazidime, cefoperazone and doxycycline. Transferable drug resistance plasmid carrying rates of these clinical isolates were also studied. On the basis of the in vitro activities, 52.63%(30/57) of the isolated strains of P. aeruginosa were susceptible to antimicrobial agents selected (except doxycycline), 41.67%(15/36) of the isolated strains of Acinetobacter were susceptible to 11 antimicrobial agents. The sensitivity rate of P.aeruginosa and Acinetobacter to antimicrobial agents selected was 70% or greater to all except doxycycline. Furthermore, the sensitivity rate of P.aeruginosa to amikacin ciprofloxacin, ceftazidime, cefoperazone, cefoperazone/sulbactam, and that of Acinetobacter to cefoperazone/sulbactam, amikacin was more than 90%,among them amikacin, cefoperazone/sulbactam being the most effective. Plasmid analysis showed that 15.79%(9/57) P.aeruginosa strains and 13.89%(5/36) Acinetobacter strains carried plasmid. Conjugative plasmid carrying rates of P. aeruginosa strains and Acinetobacter strains were 7.02%(4/57), 13.89%(5/36), respectively. Conjugative plasmid didn′t play an important role in the formation and dissemination of drug resistance of P. aeruginosa and Acinetobacter.

Pathogenic effects of biofilm with chronic pseudomonas aeruginosa lung infection in rats

Objective： To establish an animal model of P.aeruginosa biofilm associated with chronic pulmonary infection and investigate the pathogenic effects of biofilm. Methods： Experiments in vitro, measuring the MICS, MBCS of levofloxacin（LFX）, ceftazidime（CAZ） in PAO579 in alginate beads and planktonic PAO579. Rats were challenged with 0.1 ml of PAO579（109CFU/ml） in alginate beads or 0.1 ml of planktonic PAO579（109CFU/ml）, 3,7,14 days after challenging, bacteriological, pathological features were observed. Results： The MICS, MBCS of LFX, CAZ in PAO579 in alginate beads were higher than those in planktonic PAO579 in vitro. CFU/lung in alginate beads group was significantly higher than that in planktonic bacteria group（P = 0.002, P = 0.004, P = 0.002, respectively）; macroscopic lung pathology and the inflammation in alginate beads group were significantly more severe compared to those in planktonic bacteria group in vivo. Conclusion： P.aeruginosa biofilm protected bacterium from killing of antibiotics and might mediate the host immune damage in the lung tissue and made bacterium evade the host immune defense.

Isolation, identification and characterization of cadmium-resistant Pseudomonas aeruginosa strain E_1

Strain E1 with resistance to 18 mmol/L cadmium (Cd), isolated from Cd-contaminated soil was identified by morphological observation, biochemical and physiological characterization and 16S rDNA sequence analysis. The resistance to heavy metals Cd, Cu, Co, Mn, Pb, Zn and 12 antibiotics was examined. The ability of removing Cd from solution was studied. The characterizations show that strain E1 is affiliated to Pseudomonas aeruginosa (P. aeruginosa). Strain E1 has high resistance to heavy metals and the order is found to be Cd>Mn>Zn>Cu>Pb>Co in solid media. Strain E1 also exhibits the resistance to 12 antibiotics. Both living and non-living cells of strain E1 can remove Cd from solution, and living cell has better biosorption than non-living cell.

EFFECTS OF RADIX ANGELICAE SINENSIS AND SHUANGHUANGLIAN ON A RAT MODEL OF CHRONIC PSEUDOMONAS AERUGINOSA PNEUMONIA

Objective. To study the effects of two kinds of Chinese herbal medicine, Radix angelicae sinensis(RAS)(当归)and Shuanghuanglian(SHL)(双黄连) on chronic Pseudomonas aeruginosa(PA)lung infection in a rat model mimicking cystic fibrosis(CF). Methods.Rats were divided into RAS, SHL and control groups. All rats were challenged intratracheally with alginate embedded PA and the treatments with herbal medicine started on the same day of challenge. The drugs were administered subcutaneously once a day for ten days and the control group was treated with sterile saline.The rats were sacrificed two weeks after challenge. Results. Significantly improved lung bacterial clearance(P<005, P<001) and milder macroscopic lung pathology (P<0005) were found in the two treated groups compared to the control group. In the SHL treated group, the neutrophil percent in the peripheral blood leukocytes(P<005), the antiPA IgG level in serum (P<005), the incidence of lung abscesses(P<0005) and the incidence of acute lung inflammation(P<005) were significantly lower than in the control group. The RAS treatment reduced fever(P<005), decreased the incidence of lung abscesses(P<0005) and lung mast cell number (P<005), and lowered antiPA IgG1 level in serum(P<005) when compared to the control group. The antiPA bacterial activity test in SHL was weakly positive whereas in RAS it was negative. Conclusion.The treatment with both herbal medicines could increase the resistance of the rats against PA lung infection and they therefore might be potential promising drugs for stimulation of the immune system in CF patients with chronic PA lung infection.

A Modified Selective Medium Containing Benzalkonium Chloride (BKC) for the Isolation of <i>Pseudomonas aeruginosa</i>from Raw Milk

A modified selective medium (modified Cetrimide Agar, mCA) consisting of 200 μg/mL benzalkonium chloride (BKC) was developed for the isolation of Pseudomonas aeruginosa from raw milk. Initially, a total of 55 isolates were obtained from 14 raw milk samples collected from several dairy plants in Ankara, Turkey. Among these isolates, 19 were identified as Pseudomonas aeruginosa, 28 as Pseudomonas fluorescens, 4 as Acinetobacter baumannii, 2 as Enterobacter intermedium, 1 asEnterobacter agglomerans, and 1 as Escherichia coli using Microbact biochemical test kit. BKC was chosen as a selective agent to suppress growth of competitive flora because it is very effective against a wide range of Gram-negative bacteria while P. aeruginosa is resistant. MICs (minimum inhibitory concentration) for BKC were determined by agar dilution method. The concentration of 200 μg/mL BKC inhibited competitive flora, while 90% of P. aeruginosa strains were resistant. When the results of enumeration of P. aeruginosa and other Gram (-) bacteria in Cetrimide Agar (CA) and mCA were compared, it was observed that mCA was more selective than the standard CA in preventing the growth of competitive flora especially of P. fluorescens.

Prevalence and Resistance Pattern of <i>Pseudomonas aeruginosa</i>Isolated from Surface Water

Pseudomonas aeruginosa is one of the most common pathogenic bacteria, frequently found in different environmental samples. The prevalence of multidrug resistant isolates has become an alarming concern for both patients and their surroundings. The present study was carried out to record prevalence of P. aeruginosa in surface water of Dhaka city and to screen their antibiotic resistance pattern. The study was also extended to typing of resistant isolates according to extended spectrum beta lactamase production. Hereby, Kirby-Bauer method was applied to test antibiotic sensitivity according to Clinical and Laboratory Standards Institute. Then, the Ampicillin resistant isolates were screened for ESBL production by Double Disk Synergy Test (DDST). In these prospects, 52 water samples were tested, of which 32 were found positive for P. aeruginosa isolates. Hundred percent of the positive isolates were found to Ampicillin (AMP) resistant followed by 93.7% to both Tetracycline and Gentamycin and 71.8% to Co-triimoxazole. P. aeruginosa is completely susceptible to third generation antibiotics ciprofloxacin, Imipenem and Aztreonam followed by moderately susceptible to Polymyxin-B (78.2%) and Colistin (87.5%). According to DDST, all of the susceptible isolates were found positive for AMC type beta-lactamase production. It is evident from this study that the surface water is contaminated with antibiotic resistant P. aeruginosa and that through the water systems antibiotic resistance can be transferred to humans and animals. So, appropriate and rationale use of antibiotic should be applied to minimize the emergence of multidrug isolates to environment.

Development of a Duplex Real-Time PCR Method for the Pharmaceutical Rapid Microbial Detection of <i>Staphylococcus aureus</i>and <i>Pseudomonas aeruginosa</i>

Objective: To develop a duplex real-time PCR assay for pharmaceutical rapid microbial detection of Staphylococcus aureus and Pseudomonas aeruginosa. Methods: The specific primers and probes were designed to amplify the femB gene of S. aureus and the DNA gyrase subunit B gene of P. aeruginosa. The sensitivity of the system was detected by a multiple proportional dilution method. In order to examine the specificity of the system, other twenty-one bacteria strains were assayed simultaneously. Results: A highly sensitive and specific duplex real-time PCR assay for the detection of S. aureus and P. aeruginosa was established. The sensitivity was 50 copies/μL. The specificity was 100%. The whole detection procedure can be finished within 2.5 h. Conclusion: The duplex real-time PCR method is efficient in detecting with good sensitivity and specificity. There is a good prospect of this method applying in disease prevention and pharmaceutical industry due to the simultaneous detection of two pathogens.

Resistance Trends among <i>Pseudomonas aeruginosa</i>Isolates in a Tertiary Care Centre in South Gujarat

It is necessary to determine the susceptibility pattern of clinical isolates especially nosocomial one in the clinical settings for making strategy for effective empirical treatment & to reduce incidence of multidrug resistant bugs. Aim of this study was to detect the antimicrobial susceptibility pattern of P. aeruginosa isolates from clinical samples between January 2014 to December 2015, received at department of Microbiology, GMC, Surat. Clinical isolates were confirmed as P. aeruginosa by phenotypic methods/Vitek2 compact system as per availability. Genetic sequencing could not be performed due to unavailability. Antimicrobial susceptibility tests were performed by Kirby-Bauer disc diffusion method/Vitek2 compact system & Interpretation was done according Clinical and Laboratory Standards Institute (CLSI) of that year [1] [2]. Seven hundred fifty seven P. aeruginosa strains were studied during the study period. Most of the isolates were from surgery ward (62%), followed by orthopaedic ward (15%). 65% of the total isolates were from swab samples followed by urine (7%), pus, fluid (5%) & devices (4%). 60% isolates were resistant to Ceftazidime & for other drugs resistance pattern was as follows: Cefepime (52%), Levofloxacin (49%), Ticarcillin/clavulanic acid (49%), Meropenem & Gentamycin (44%), Ciprofloxacin (43%), Amikacin (41%), Tobramycin (39%), Netlimycin (36%), Piperacillin (32%), Aztreonam (31%), Piperacillin/tazobactam (26%), Imipenem (23%) , Doripenem (12%) & Gatifloxacin (10%). As there is predominance of isolates from surgical ward in present study & resistance to carbapenem group of drugs was also found, indicating that most of the infection caused by Pseudomonas aeruginosa may be nosocomial.

Serotypes, Antibiogram and Genetic Relatedness of <i>Pseudomonas aeruginosa</i>Isolates from Urinary Tract Infections at Urology and Nephrology Center, Mansoura, Egypt

Background: Pseudomonas aeruginosa (P. aeruginosa) is an opportunistic pathogen that represents a major problem in many hospitals because of its increased resistance to antibiotics and the ability to cause nosocomial infections. The present study aimed to phenotype and genotype isolates of P. aeruginosa from inpatients with UTIs at Urology and Nephrology center, Mansoura, Egypt to study their relatedness. Methods: Thirty nine isolates of P. aeruginosa were phenotypically typed by determination of O-serotypes by slide agglutination technique and antimicrobial resistance patterns by disk-diffusion method. The genetic diversity of isolates was illustrated by performing RAPD-PCR using M13 primer. Results: Serotypes O11, O6 and O10 were the most prevalent. Isolates showed high resistance rates to antipseudmonal antibiotics with high incidence (51.3%) of multidrug resistance (MDR). Amikacin was the most effective. A significant correlation was found between O6, O10 and MDR. A relatively high polymorphism was demonstrated among P. aeruginosa isolates by using RAPD-M13 fingerprinting. Cross transmission was suggested by phenotypically and clonally identical isolates. Conclusion: The study demonstrates the role of combining both classical and molecular typing as a valuable mean to study the origin and cross transmission of P. aeruginosa in UTIs for better assessment of treatment and infection control.

Impact of Sulfidation of Silver Nanoparticles on Established<i>P. aeruginosa Biofilm</i>

Silver nanoparticles (Ag-NPs), one of the most common types of nanomaterials in medical fields and consumer products, are known to have antimicrobial effects;these materials also undergo a series of chemical and biological transformations in the environment. Although the pristine form of silver nanoparticles has been studied, less is known about the impacts of the transformed Ag-NPs on biological systems. This knowledge gap hinders the progress of effectively assessing the impacts of Ag-NPs on the environment and human health. In this study, we demonstrate that the most common form of transformed Ag-NPs, sulfidized silver nano-particles (Ag2S-NPs), show less damage on established Pseudomonas aeruginosa GFP (ATCC? 10145 GFP?) biofilm than the pristine form of the nanoparticle. At a dosage of 0.625 mg/L, the total biomass in the biofilm decreased 64% after being exposed to Ag-NPs and 44% after exposure to Ag2S-NPs. Live biofilms were also interrogated. We observed high reduction in live population for biofilm exposed to Ag-NPs and relatively low reduction by Ag2S-NPs at exposure concentrations higher than 0.625 mg/L. Compared with Ag-NPs, the lower solubility of Ag2S-NPs results in less Ag+ diffusion into established biofilms. Our results suggest that the sulfidation of Ag-NPs reduces their impacts on established biofilms, indicating that the transformed Ag-NPs may have less environmental or human health risks.

Expression of IL-4 in a rat model of chronic pulmonary infection with biofilm formation induced by Pseudomonas aeruginosa

<正>The expression of IL-4 in a rat model of chronic pulmonary infection biofilm formation induced by Pseudomonas aeruginosa was investigated,in which SPF Wister rats were infected via trachea with 0.1 ml P.aeruginosa strain PAO579(10~9 CFU/ml)in alginate beads or the planktonic form of this bacterial strain(10~9 CFU/ml),and on 3,7 and 14 d after infection,the bacteriological and pathological changes were observed as well as the expression of the cytokine IL-4 was determined.It was demonstrated that the count of CFU per lung tissue in case of bacteria in alginate beads was significantly higher than that of bacteria in planktonic form,with more severe gross pathologic changes and inflammatory reactions in the alginate bead group in comparison with that of the planktonic forms(P=0.002,P=0.004 and P=0.002,respectively).In addition,the expression of IL-4 in the alginate bead group was also higher than that in the planktonic form(P=0.02,P=0.02 and P=0.022,respectively).A positive corre- lation between the level of IL-4 expression and the gross lung pathology in alginate bead group existed as demonstrated by simple regression analysis(r=0.78,P<0.02).It is concluded that the chronic pul- monary infection with biofilm formation induced by P.aeruginosa tends to have the priority to the Th2 immune response.

鱼腥草素钠对铜绿假单胞菌生物被膜藻酸盐合成的影响

目的研究鱼腥草素钠对铜绿假单胞菌ATCC27853生物被膜藻酸盐合成及相关基因的影响。方法倍比稀释法测定鱼腥草素钠对铜绿假单胞菌ATCC27853的最小抑菌浓度(MIC),对羟基联苯溶液显色法测定鱼腥草素钠干扰铜绿假单胞菌ATCC27853生物被膜生长过程中藻酸盐的产生量;扫描电镜观察生物被膜形态变化;荧光显微镜下观察膜分散后死活细菌;RT-PCR测定经鱼腥草素钠干预后的3日龄铜绿假单胞菌生物被膜菌藻酸盐合成基因algD、al-gG,调节基因algZ、algR的表达情况。结果经2×MIC鱼腥草素钠干预后藻酸盐产生量明显下降,与阴性对照组相比差异显著(P<0.05),镜下观察到细菌死亡数增多,未观察到生物被膜;藻酸盐调节基因algZ、algR与合成基因algD、algG表达水平下降,与阴性对照组相比P<0.05。结论鱼腥草素钠通过下调藻酸盐合成相关基因的表达抑制藻酸盐产生,进而干扰铜绿假单胞菌生物被膜的形成。

鱼腥草素钠对铜绿假单胞菌生物被膜的清除作用

目的研究鱼腥草素钠对铜绿假单胞菌早期生物被膜及成熟期生物被膜的清除作用。方法用96孔板建立体外铜绿假单胞菌生物被膜,给药24 h后MTT法检测生物被膜最低清除浓度(sessile minimal eradicating concentration,SMEC),扫描电镜下观察药物对生物膜形态影响。结果鱼腥草素钠对铜绿假单胞菌生物被膜的SMEC50,早期是15.6 mg/L,成熟期是250 mg/L,在早期生物被膜向成熟生物被膜发展过程中SMEC50均在250 mg/L,镜下观察250mg/L药物质量浓度能清除大部分的生物被膜,同时可使铜绿假单胞菌发生形态变异。结论鱼腥草素钠对早期及成熟期的生物被膜有一定的清除作用,对早期生物被膜的清除作用更强于成熟期生物被膜。

不同质量浓度的磷对铜绿微囊藻生长及细胞内磷的影响

通过室内模拟的方法研究了在磷质量浓度不同的水体条件下,在铜绿微囊藻水华形成过程中微囊藻的增殖特征及细胞内磷、可溶性磷的变化特征。在模拟的太湖水体中,随着外源磷的增加,藻生长最终限制因素由磷限制(ρ(TP)≤0 045mg L)发展到光限制(ρ(TP)≥0 445mg L),而ρ(TP)=0 445mg L是微囊藻最适生长浓度;同时,微囊藻细胞内磷含量(QP)、水体可溶性磷(DTP)也随藻类生长而发生变化,在水体ρ(TP)<0 445mg L时,细胞内磷对微囊藻增殖有促进作用,而在ρ(TP)>0 445mg L的水体中,磷对微囊藻增殖有抑制作用。

氮磷比对水华蓝藻优势形成的影响

通过批量培养实验研究了不同磷水平下N/P比对铜绿微囊藻(蓝藻)和斜生栅藻(绿藻)生长速率的影响,并在太湖蓝藻水华暴发期间,监测了梅梁湾和湖心区水体叶绿素a浓度和氮磷营养盐结构变化,以探讨N/P比对蓝藻优势形成的影响.结果表明,N/P比对铜绿微囊藻和斜生栅藻生长的影响并不表现在一个确定值上,而与水体氮磷的绝对浓度有关,在0.02mg/L磷浓度下,铜绿微囊藻和斜生栅藻在N/P比为4:1～32:1范围内生长速率均较低(0.067～0.074,0.018～0.022d-1),说明受到营养盐的限制;当磷浓度达到0.20mg/L时,铜绿微囊藻在N/P比为32:1时生长速率达到最大值(0.240d-1),斜生栅藻在N/P比为64:1时生长速率达到最大值(0.380 d-1);而在磷浓度升高到2.00mg/L时,不同N/P比下铜绿微囊藻和斜生栅藻均达到最大生长速率(0.24～0.25,0.378～0.381d-1),说明氮磷浓度均比较充足,N/P比对生长速率已经没影响.可见,氮磷浓度比N/P比对两种藻的生长影响更大.与斜生栅藻相比,铜绿微囊藻对氮磷营养的生理需求和最大生长速率均相对较低,属K策略物种,易在低氮磷浓度下形成优势.梅梁湾在水华暴发期间氮浓度一直远低于水华较轻的湖心区,而磷浓度远高于湖心区,进而导致梅梁湾N/P质量比(低于20:1)在水华期间一直低于湖心区(124:1),低N/P比是蓝藻水华暴发导致氮浓度下降,磷浓度升高的结果.

南京地区铜绿假单胞菌的整合子流行性调查

目的调查南京地区铜绿假单胞菌的整合子流行情况,并分析整合子与铜绿假单胞菌耐药的相关性。方法收集98株南京地区临床分离的铜绿假单胞菌,K-B法测定其药敏情况,简并引物PCR法扩增整合子的整合酶基因,对阳性PCR产物采用HinfⅠ内切酶作限制片段长度多态性(RFLP)分析进行整合子分类。结果98株铜绿假单胞菌对哌拉西林等14种抗菌药的耐药率从14.3%到82.7%。40.8%(40/98)的铜绿假单胞菌中检出整合子;PCR-RFLP结果显示均为Ⅰ类整合子,未检出Ⅱ类和Ⅲ类整合子。结论Ⅰ类整合子较广泛地存在于南京地区铜绿假单胞菌中;整合子与铜绿假单胞菌的耐药和多重耐药具有相关性。

氮磷比例对铜绿微囊藻生长及部分生化组成的影响

对在不同N/P(1∶1,5∶1,16∶1,50∶1,100∶1)培养条件下,铜绿微囊藻的生长和营养生理特征进行了研究。结果表明,在N/P=16∶1的条件下,铜绿微囊藻的生长速度最快,细胞生物量最高;N/P小于16时,铜绿微囊藻的生长状态较N/P大于16时好,说明其生长主要受磷的限制。藻细胞碳水化合物的含量也受N/P的影响,其含量表现为16∶1>5∶1>1∶1>50∶1>100∶1;此外,藻细胞叶绿素含量随N/P的增加而降低。

氮磷对微囊藻和栅藻生长及竞争的影响

为了揭示不同营养条件下,藻类优势种的形成规律,选取了3种具有代表性水体的营养盐浓度,对于蓝藻水华的常见种铜绿微囊藻和绿藻水华的常见种四尾栅藻进行了竞争实验.通过竞争抑制参数对相互间的竞争关系进行了分析.结果表明,在贫营养水平下,栅藻的存在能够刺激微囊藻的生长,N/P值越小,刺激作用越明显,微囊藻也能刺激栅藻的生长;富营养水平下,竞争抑制作用与N/P有关;超富营养水平下,栅藻对微囊藻的抑制能力约为微囊藻对栅藻的抑制能力的3倍,N/P值的变化对竞争抑制作用的影响不明显.在较低氮磷浓度的水体中,微囊藻容易成为优势种,而在较高的氮磷浓度的水体中,四尾栅藻更容易成为优势种.