大肠酶对猪饲料酶水解物能值的影响及与非淀粉多糖组分的关系

【目的】研究大肠酶对单胃动物仿生消化系统测试猪饲料原料的体外干物质消化率(DMD)和酶水解物能值(EHGE)的影响,并分析不同大肠酶条件下非淀粉多糖(NSP)组分与DMD和体外总能消化率(GED)的关系,为完善体外模拟胃-小肠-大肠三步消化方法提供参考依据。【方法】采用单因素完全随机设计,共设4个处理,在单胃动物仿生消化系统模拟饲料原料胃和小肠消化后,分别使用对照组(去离子水)、纤维素酶、Viscozyme酶和仿生酶(由纤维素酶、木聚糖酶、β-葡聚糖酶和果胶酶组成)模拟大肠阶段的消化。每个处理设5个重复,每个重复1根消化管,分别测定玉米、大豆粕、小麦麸、玉米DDGS、苜蓿草粉和大豆皮的DMD、GED和EHGE。并使用乙酸酐衍生化气相色谱法测定6种饲粮原料NSP含量和组分。分析饲料原料NSP组分与DMD及GED的相关关系。【结果】(1)在对照组中,玉米的DMD最高,达到了81.51%,相应的EHGE为15.39 MJ·kg^(-1),而大豆皮的DMD最低,只有10.60%,相应的EHGE只有2.42 MJ·kg^(-1)。(2)3种模拟大肠酶均显著提高了玉米、大豆粕和大豆皮的DMD(P<0.01),提高了大豆粕和大豆皮的EHGE(P<0.01)。但纤维素酶作用下苜蓿草粉、玉米DDGS的DMD和EHGE与对照组差异不显著,Viscozyme酶作用下小麦麸、玉米DDGS的DMD和EHGE与对照组差异不显著(P>0.05)。仿生酶显著提高了6种饲料原料的DMD(P<0.01),显著提高了除玉米DDGS外的其他5种饲料原料的EHGE(P<0.01)。(3)不同的大肠酶对不同饲料原料体外消化率的提升程度不同。在6种原料中,纤维素酶对小麦麸的DMD和EHGE提升程度最高,分别达到了5.89%和1.03 MJ·kg^(-1),而只使大豆粕的DMD和EHGE提高了1.26%和0.36 MJ·kg^(-1);Viscozyme酶对大豆皮体外消化率的提升程度最高,分别使其DMD和EHGE提高6.01%和1.02 MJ·kg^(-1)。仿生酶对小麦麸的DMD和EHGE的提升程度最高,达到了6.59%和1.37 MJ·kg^(-1)。(4)6种饲料原料的可溶性非淀粉多糖(SNSP)的含量均低于不溶性非淀粉多糖(INSP),玉米的总非淀粉多糖(TNSP)含量最低(8.59%),大豆皮的TNSP含量最高(75.72%),各原料的NSP主要由阿拉伯糖、木糖、甘露糖和葡萄糖组成,但不同原料中4种单糖含量存在差异。(5)6种饲料原料的SNSP、INSP以及TNSP含量与DMD、GED均呈显著的负相关(P<0.05)。仿生酶作用下DMD与TNSP含量的相关性(R^2=0.95,P<0.01)高于纤维素酶(R^2=0.94,P<0.01)和Viscozyme酶(R^2=0.93,P<0.01)。同时,仿生酶作用下GED与TNSP含量的相关性(R^2=0.89,P<0.01)也高于纤维素酶(R^2=0.86,P<0.01)和Viscozyme酶(R^2=0.81,P<0.01)。【结论】仿生酶在体外模拟猪大肠消化过程中,对饲料的消化作用优于纤维素酶和Viscozyme酶,可作为单胃动物仿生消化系统体外模拟猪消化中大肠阶段的模拟消化酶。

大肠杆菌丙酮酸脱氢酶的克隆与表达优化

为了在大肠杆菌中表达大肠杆菌丙酮酸脱氢酶,用PCR法从大肠杆菌总DNA中克隆了pdc基因,将其插入载体pGEX-KG后转化大肠杆菌BL21(DE3),在IPTG的诱导下实现了表达。通过对表达条件的优化,在TB+M9(1∶1)培养基中,33℃下使用终浓度0.5 g.L-1的乳糖诱导4 h,重组大肠杆菌丙酮酸脱氢酶的表达量可占全菌蛋白的45%左右,比未优化前提高了约20%,同时大大降低了成本。

社区及医院感染大肠埃希菌产AmpC酶、ESBLs检测与耐药性分析

目的探讨引起社区和医院感染的大肠埃希菌产AmpC酶、超广谱β-内酰胺酶(ESBLs)情况及其对常用抗菌药物的耐药性,以指导临床合理选择抗菌药物。方法采用头孢西丁酶提取物三维试验测定AmpC酶;双纸片协同试验和纸片确证试验筛选并确认产ESBLs菌株。结果143株大肠埃希菌产AmpC酶、ESBLs及AmpC酶+ESBLs的总检出率分别为4.90%、28.67%、2.10%。非产酶株总耐药率,医院感染株为35.36%,社区感染株为21.85%,两者比较,差异有显著性(P<0.05);产酶株总耐药率两者分别为73.40%、75.60%,差异无显著性(P>0.05)。社区和医院感染的非产酶菌株对氨苄西林、哌拉西林、头孢唑林、环丙沙星等常用抗菌药物都有较高的耐药率,分别为57.58%、39.39%、42.42%、39.39%及77.97%、71.19%、66.10.%、54.24%;产酶菌株的耐药率均高于上述平均水平。所有被测药物中,亚胺培南/西司他丁敏感性最高,未出现耐药株。结论社区感染的大肠埃希菌非产酶株耐药率明显低于医院感染株。大肠埃希菌耐药的主要原因是产ESBLs和AmpC酶;亚胺培南/西司他丁为目前大肠埃希菌产酶株感染的临床经验首选用药。

转大肠杆菌过氧化氢酶基因棉花的抗旱生理研究

以导入大肠杆菌过氧化氢酶基因KatE的T3代转基因棉花为供试材料,经卡那霉素检测和PCR鉴定,将筛选出的阳性转基因植株与对照棉花进行整个生育期的持续水分胁迫处理直至收获,比较材料间的生理生化指标的差异,鉴定转基因植株的耐旱能力。结果显示:(1)干旱胁迫持续至初蕾期时,转基因棉花与对照植株间各项抗旱生理指标差异均未达到显著水平。(2)水分胁迫持续至盛蕾和盛花期时,转基因棉花叶片相对含水量、光系统Ⅱ最大光化学效率(Fv/Fm)、CAT活性,以及叶片的净光合速率(Pn)、气孔导度(Gs)和蒸腾速率(Tr)均显著或极显著高于对照植株,叶绿素含量也都明显高于对照植株。干旱胁迫持续至吐絮期时,转基因棉花的株高、果枝数和铃数均显著或极显著高于对照植株,且转基因棉花和对照的籽棉产量分别比正常灌溉处理降低57.5%和60.1%,全生育期的水分胁迫严重影响了棉花籽棉产量,但转基因棉花的籽棉产量仍显著高于对照。研究表明,在新疆石河子当地自然降水(干旱胁迫)条件下,转KatE基因棉花表现出了较好的生理和生长优势,KatE基因有助于提高棉花的抗旱性。

藤黄微球菌过氧化氢酶基因在大肠杆菌中的重组与表达

目的应用基因重组技术在大肠杆菌中高效表达藤黄微球菌过氧化氢酶(catalase,CAT)。方法从藤黄微球菌DNA中获得CAT编码基因,并应用pProEx-HTa质粒构建融合表达载体并表达和检测活性。结果通过融合表达获得可溶性带6×His标签重组蛋白,该蛋白经过Ni-NTA纯化后可获得活性物质。结论从大肠杆菌表达体系中表达了具有生物活性的CAT。

1例产酶大肠埃希杆菌的用药监护

目的研究产酶大肠埃希杆菌感染的治疗方法和用药监护。方法对1例肺病感染患者进行病例跟踪,分析更换抗生素的原因,总结使用不同抗生素的使用效果。结果长期使用三代头孢,使产酶大肠埃希杆菌的耐药性增加,但对复合三代头孢仍较敏感。结论随着产酶大肠埃希杆菌耐药性的逐年递增,其抗生素的治疗应做药学监护。

小檗碱联合头孢他啶对产AmpC酶大肠埃希菌体外抑制作用研究

目的:探讨小檗碱联合头孢他啶对产AmpC酶大肠埃希菌体外的抑制作用,为临床中西医结合治疗提供用药依据。方法:分别检测小檗碱和头孢他啶对20株产AmpC酶大肠埃希菌株的MIC;采用K-B法对20株产AmpC酶大肠埃希菌做单独小檗碱、单独头孢他啶及头孢他啶+小檗碱的联合药敏试验。结果:头孢他啶对产AmpC酶大肠埃希菌MIC 8~256 g/L;小檗碱对产AmpC酶大肠埃希菌MIC 31.25~250 g/L;头孢他啶+小檗碱联合药敏试验对耐药菌FIC表现均为相加作用;20株产AmpC酶大肠埃希菌药敏试验表现为头孢他啶联合小檗碱比单用头孢他啶的药敏抑菌环直径增大,差异有统计学意义(P<0.05)。结论:小檗碱对产AmpC酶大肠埃希菌具有抑制作用;小檗碱联合头孢他啶对产AmpC酶大肠埃希菌联合药敏结果呈相加作用。

头孢他定与头孢噻肟对泌尿系产超广谱β-内酰胺酶的大肠埃希菌检出率分析

目的:了解头孢他定(Ceftazidime,CAZ)和头孢噻肟(Cefotaxime Sodium,CTX)对我院引起泌尿系感染的大肠埃希菌(Escherichia coli,ECO)产超广谱β-内酰胺酶(extended-spectrumβ-lactamase,ESBLs)菌株的体外检出特点,以更好的筛选出高度耐药菌株,避免漏检。方法:用K-B纸片筛选及确证试验,对126株大肠埃希菌(ECO)进行产超广谱β-内酰胺酶(ESBLs)检测分析。结果:头孢噻肟对产ESBLs的ECO检出率为93.10%、头孢他定对产ESBLs的ECO检出率为44.83%。结论:头孢噻肟对产ESBLs的ECO检出率显著高于头孢他定对产ESBLs的ECO检出率。

Mecillinam和羟氨苄青霉素/克拉维酸对产酶大肠杆菌的体外活性

Mecillinam(MPC)是6-β-脒基青霉酸衍生物。它通过优先与青霉素-结合蛋白2相结合而发挥其抗菌作用。结果在形成球状细菌细胞中其杀菌作用较其它抗生素更佳。本文旨在研究大肠杆菌产生的β-内酰胺酶是否足以导致对MPC耐药,以及不同的β-内酰胺酶是否对MPC耐药的影响亦不同。为了便于比较同时做了羟氨苄青霉素(AMPC)/克拉维酸(CV A)联用试验。用标准方法研究并鉴别产生TEM-1(RichmondⅢa型),Oxa-1(RichmondⅤ型)和染色体介导β-内酰胺酶(RichmondⅠ型)的大肠杆菌临床分离菌株,这些菌株均为最普遍的对氨苄青霉素族耐药(MIC大于64μg/ml)

渗透剂对苹果酸脱氢酶包含体的复性作用

将甜菜碱和海藻糖两种渗透剂作为添加剂,考察了其促进苹果酸脱氢酶包含体的复性作用。结果显示,甜菜碱和海藻糖均可有效促进大肠杆菌苹果酸脱氢酶包含体的复性。在本文实验条件下,随添加甜菜碱浓度的升高,复性后苹果酸脱氢酶的比活增大;而海藻糖则出现最佳添加浓度使复性后苹果酸脱氢酶的比活最大;同时在盐酸胍浓度较高、不添加渗透剂时复性效果较差的复性体系中,若添加合适浓度的甜菜碱或海藻糖即可有效促进苹果酸脱氢酶的复性,显示出渗透剂作为添加剂在实际包含体蛋白质复性过程中的应用前景。另外,通过外源荧光分析发现,添加甜菜碱和海藻糖均可降低苹果酸脱氢酶表面疏水性区域的暴露程度;圆二色光谱分析则表明,甜菜碱和海藻糖可以促进苹果酸脱氢酶α-螺旋结构的生成。

CCA培养基同时检测水中总大肠菌群和大肠埃希氏杆菌

大肠菌群(Coliforms)和大肠埃希氏杆菌(E.coli)都是判断水体是否存在粪便污染的重要微生物指标。本文介绍了一种可在24h之内同时检测大肠菌群和大肠埃希氏杆菌数量的CCA培养基。

Molecular Cloning, Escherichia coli Expression and Genomic Organization of Squalene Synthase Gene from Artemisia annua

A 1 539 by squalene synthase (AaSQS) cDNA was cloned from a high-yield Artemisia annua L. strain 001 by reverse transcription-polymerise chain reaction (RT-PCR). The amino acid sequence of AaSQS is 70%, 77%, 44% and 39%a identical to that of squalene synthases from Arabidopsis thaliana, tobacco, human and yeast, respectively. The AaSQS genomic DNA has a complex organization containing 14 exons and 13 introns. Full-length or C-terminal truncated cDNA was subcloned into prokaryotic expression vector pET30a and the constructed plasmid was introduced to Escherichia coli strain BL21 (DE3) for induced overexpression. No squalene synthase protein with expected molecular mass was observed in E. cola containing the putative full-length squalene synthase cDNA, however, overexpression in E. coli was achieved by truncating 30 amino acids of hydrophobic region at the carboxy terminus.

产AmpC酶大肠埃希菌中整合子的研究

目的:观察25株产AmpC酶大肠埃希菌中整合子的分类、结构及其在介导AmpC酶基因转移中的作用。方法:采用微量稀释法测定20种抗生素对试验菌株的敏感性。利用多重聚合酶链反应(PCR)方法检测整合酶基因(intI)及其定位,对其阳性菌株可变区(Int)扩增产物进行测序分析。结果:这25株菌对多种抗生素耐药。20株Ⅰ类整合酶基因阳性(80%);所携带的耐药基因盒绝大多数为aadA5和dfr17;未发现携带AmpC基因盒的整合子。结论:Ⅰ类整合子广泛地存在于产AmpC酶的大肠杆菌中;耐药基因盒是整合子阳性菌株对氨基糖苷类、磺胺类药物及氯霉素耐药的主要原因,但对介导AmpC酶基因转移,不起主要作用。

Study on the Resistance of Pathogenic Escherichia coli to Ceftiofur

[Objective] Ceftiofur was as the substrate to induce the standard strain of Escherichia coli（E.coli）to be the drug-resistance one.The resistant mechanism of E.coli to ceftiofur was studied.[Method] The sub-inhibitory concentration method was used to induce the standard strains C83907 and C83845.After they were induced for 10 generations,the double disc synergy test（DDST）,NCCLS（National Committee for Clinical Laboratory Standards）confirmatory test and PCR amplification were used to detect the extend spectrum β-lactamases（ESBLs）.The two fold dilution method was used to measure the minimal inhibitory concentration（MIC）of cetiofur to the strain which produced ESBLs.For the drug-resistance strain which produced ESBLs,the two fold dilution method was used to measure the minimal inhibitory concentrations of different proportions of cetiofur and tazobactam sodium.[Result] After they were induced 15 generations,MIC value of ceftiofur to the induced bacteria was during 8-10 μg/ml,and ESBLs was detected.MICs of cetiofur combining tazobactam sodium（the mass ratio was 1∶1-8∶1）to Escherichia coli produced ESBLs reduced 20-22 times than that of cetiofur.[Conclusion] The main mechanism of pathogenic Escherichia coli resistance to ceftiofur was that which produced ESBLs.

大肠杆菌磷酸甘油酸脱氢酶突变体的构建及抗反馈抑制效应

磷酸甘油酸脱氢酶(D-3-phosphoglycerate dehydrogenase,PGDH,EC 1.1.1.95)为L-丝氨酸合成途径的关键酶,其编码基因为ser A,其活性受到合成产物L-丝氨酸的反馈抑制调控。为解除丝氨酸的反馈抑制,采用定点突变技术把编码PGDH酶344位组氨酸或346位天冬氨酸或364位天冬氨酸的密码子定点突变为丙氨酸密码子。改造后的ser AFbr被连到表达载体pT7-7上,并转入大肠杆菌Escherichia coli BL21(DE3)中进行表达,破壁回收粗酶液,通过DEAE阴离子柱纯化PGDH突变体,并对其酶活性和IC_(50)值进行了测定。结果,野生型PGDH酶IC_(50)值为7μmol/L,而PGDH双突变体N346A/H344A催化活性与野生型相近,在丝氨酸浓度为160 mmol/L时,其酶活仍保持未添加丝氨酸时酶活的96%,基本解除反馈抑制。

Construction of Plant-based Expression Vector of Polyphosphate Kinase Gene

[Objective] The aim was to construct the fusion expression vector of polyphosphate kinase（PPK） and green fluorescent protein（GFP） genes.[Method] In this study,the primers were designed based on PPK gene sequence（L03719） of E.coli DH5α in Genbank.Genomic DNA of E.coli DH 5α was extracted as template for the amplification of PPK gene by PCR method.By using In-Fusion@ HD Cloning Kit,the PPK gene was directionally cloned into NcoI site of the pCAMBIA1302 vector.[Result] Sequencing results showed that the 2.0 kb long fragment of PPK gene was inserted into the plant-based expression vector pCAMBIA1302 in front of GFP gene.[Conclusion] The fusion expression vector of PPK and GFP genes were successfully constructed.

Cloning of Endo-β-Glucanase Ⅲ and Expression in Eerevisiae Fermentum

Objective The aim was to construct bioengineering strains that could degrade the cellulosic solid waste. Method The cDNA of endo-β-glucanase III of Trichoderma vi ride AS313711 was cloned by RT-PCR method. After sequenced, this gene was constructed to expression vector pESP-2, and then the plasmid was transformed into competent cell of cerevisiae fermentum by electric shock, the transformant was then obtained. The enzyme activity of this transformant at the different temperatures and pH was measured by DNS method. Result The length of ORF of EG III was 1 257 bp, encoding 418 amino acids, while the deduced molecular weight was 44.1 × 103 kD. Conclusion The enzyme activity of EG III was the highest when it was at PH 4.9 and tempeture was of 60℃. Then the corresponding enzyme activity was about 100%.