亚热带人工林下植被根际土壤酶化学计量特征

为探讨林下植被根际土壤酶化学计量特征及其对林分类型和季节的响应, 该研究以江西省泰和县千烟洲试验站典型人工杉木(Cunninghamia lanceolata)、马尾松(Pinus massoniana)和湿地松(Pinus elliottii)林林下优势灌草檵木(Loropetalum chinense)、杨桐(Adinandra millettii)、格药柃(Eurya muricata)、狗脊蕨(Woodwardia japonica)和暗鳞鳞毛蕨(Dryopteris atrata)为对象, 在植被生长初期(4月)和旺盛期(7月)测定优势灌草根际土壤与碳(C)循环相关的β-1,4-葡萄糖苷酶(BG)、与氮(N)循环相关的β-1,4-N-乙酰葡糖氨糖苷酶(NAG)和亮氨酸氨基肽酶(LAP)、与磷(P)循环相关的酸性磷酸酶(AP)活性、酶化学计量比及土壤理化性质。结果发现: (1)根际土壤与C和N循环相关的酶活性以及BG:AP (酶C:P)在不同林下植被之间存在显著差异, 而与P循环相关的酶活性差异不显著。林分类型和取样季节显著影响BG:(NAG+LAP)(酶C:N), 且林下植被类型、林分类型和取样季节交互影响酶C:P。主成分分析表明, 根际土壤酶的活性及计量比在不同林下植被(檵木不同于格药柃, 且二者显著区别于其他物种)、林分类型(杉木林区别于马尾松、湿地松林)和取样季节之间均存在显著差异。土壤硝态氮(NO₃ ^--N)、铵态氮(NH₄ ⁺-N)、可溶性有机碳(DOC)含量和碳氮比(C:N)是影响林下植被根际土壤酶的活性及化学计量比的主要因素。(2)标准主轴回归分析表明, 林下植被根际土壤lg(BG)、lg(NAG+LAP)和lg(AP)之间存在显著线性关系, lgBG:lg(NAG+LAP):lgAP (酶C:N:P)约为1:1:1.3, 酶C:P及(NAG+LAP):AP (酶N:P)分别为0.14和0.15。AP远大于BG和NAG+LAP的活性, 导致lg(BG)和lg(NAG+LAP)与lg(AP)的回归斜率极显著偏离1。说明林下植被根际土壤酶的活性及计量比受植被种类、林分类型及取样季节影响, 且基质有效性在其中发挥重要作用。相较于C循环和N循环, 微生物会分配更多资源用于P循环相关酶的生产, 暗示亚热带人工林林下植被根际土壤微生物生长和活性更易受P限制。     

研究: 载脂蛋白E拟肽EpK对apoE-/-小鼠动脉粥样硬化的影响

前期设计合成了一种模拟人载脂蛋白E(apoE)结构域的小分子多肽EpK,体外实验证实该拟肽具有抑制巨噬细胞炎症及增强高密度脂蛋白(HDL)介导细胞胆固醇外流的作用．本文拟借助慢病毒体系分泌性表达EpK,研究EpK在体对apoE基因敲除(apoE^-/-)小鼠动脉粥样硬化斑块的影响．将11月龄雌性apoE^-/-小鼠18只,随机分两组,分别经眼球后静脉丛注射pWPI慢病毒(Lv-GFP对照组)和含EpK的重组慢病毒(Lv-EpK组)．小鼠普食喂养,间隔采血监测血脂状态,检测血浆对氧磷酯酶(PON1)活性,病毒注射18周后小鼠安乐死,从主动脉根部连续冰冻切片及主动脉胸腹段纵剖面(en face)进行油红O染色分析斑块面积,采用实时荧光定量PCR检测小鼠肝脏相关基因的mRNA表达水平,蛋白质印迹检测血浆中apoA-Ⅰ、PON1及血清淀粉样蛋白A(SAA)水平．结果显示：慢病毒感染小鼠可成功在血循环中检测到EpK,与Lv-GFP对照组比较,Lv-EpK组apoE^-/-小鼠的血脂及脂蛋白分布、apoA-Ⅰ水平、PON1活性无明显改变,但EpK组小鼠的主动脉斑块面积较对照组显著减少(主动脉根部斑块面积(0.87±0.07) mm² vs (1.03±0.08) mm²,P < 0.05;主动脉胸腹段斑块占管腔比42.0% vs 55.8%,P < 0.01)．EpK可显著降低血中SAA水平,并抑制肝脏炎症因子TNF?琢和IL-6的表达．结果说明,EpK拟肽具有减退apoE^-/-小鼠动脉粥样硬化斑块的作用,其机制可能与其发挥的抗炎作用有关．     

地衣芽胞杆菌FLP/FRT基因编辑系统的构建及验证

地衣芽胞杆菌有效的基因编辑工具有限,为了拓展和丰富其基因编辑手段,在地衣芽胞杆菌中构建一个抗性标记可重复使用的FLP/FRT基因编辑系统,并通过敲除α-淀粉酶基因amyL、蛋白酶基因aprE及敲入外源透明颤菌血红蛋白基因vgb对该系统进行初步验证。首先以温敏质粒pNZT1为载体分别构建amyL和aprE基因敲除质粒pNZTT-AFKF和pNZTT-EFKF,两个敲除质粒各自包含针对目标基因的同源臂、抗性基因及同向的FRT位点;将敲除质粒转化地衣芽胞杆菌并经过两次同源交换过程实现目标基因的敲除;最后导入一个FLP重组酶表达质粒通过FLP/FRT系统的重组作用介导抗性基因的回收。为进一步验证本系统的实用性及编辑效率,构建了包含透明颤菌血红蛋白编码基因vgb表达盒及基因组丙酮酸甲酸裂解酶编码基因pflB敲除盒的重组质粒pNZTK-PFTF-vgb,并以此进行外源基因vgb在基因组上的定向敲入。结果显示,成功敲除amyL及aprE并回收了抗性标记卡那霉素基因,敲除后淀粉酶活和蛋白酶活分别减少95.3%和80.4%;vgb基因成功整合入基因组pflB位点并回收了抗性标记四环素基因,并利用荧光定量PCR技术检测到vgb的整合表达。文中首次建立了一个适用于地衣芽胞杆菌的、抗性标记可重复使用的FLP/FRT基因编辑系统,并进行了基因敲除及基因敲入验证,为地衣芽胞杆菌遗传改造提供了良好的方法参考。     

Characterization of coliphage PR772 and evaluation of its use for virus filter performance testing

Virus filtration is a key clearance unit operation in the manufacture of recombinant protein, monoclonal antibody, and plasma-derived biopharmaceuticals. Recently, a consensus has developed among filter manufacturers and end users about the desirability of a common nomenclature and a standardized test for classifying and identifying virus-retentive filters. The Parenteral Drug Association virus filter task force has chosen PR772 as the model bacteriophage to standardize nomenclature for large-pore-size virus-retentive filters (filters designed to retain viruses larger than 50 to 60 nm in size). Previously, the coliphage PR772 (Tectiviridae family) has been used in some filtration studies as a surrogate for mammalian viruses of around 50 to 60 nm. In this report, we describe specific properties of PR772 critical to the support of its use for the standardization of virus filters. The complete genomic sequence of virulent phage PR772 was determined. Its genome contains 14,946 bp with an overall G+C content of 48.3 mol%, and 32 open reading frames of at least 40 codons. Comparison of the PR772 nucleotide sequence with the genome of Tectiviridae family prototype phage PRD1 revealed 97.2% identity at the DNA level. By dynamic light-scattering analysis, its hydrodynamic diameter was measured as 82 +/- 6 nm, consistent with use in testing large-virus-retentive filters. Finally, dynamic light-scattering analysis of PR772 preparations purified on CsCl gradients showed that the phage preparations are largely monodispersed. In summary, PR772 appears to be an appropriate model bacteriophage for standardization of nomenclature for larger-pore-size virus-retentive filters.     

离体条件下诱导番茄果实状结构的再生

以番茄（Ｌｙｃｏｐｅｒｓｉｃｏｎ ｅｓｃｕｌｅｎｔｕｍ Ｍｉｌｌ．）雌蕊和幼果的组织作外植体可以诱导果实状结构的再生。这种果实状结构在离体条件下能培养成熟,成熟时具红色。解剖观察表明：果实状结构由果肉和包围在外面的果皮组成,无种子和胎座。外源激素和外植体年龄的试验揭示：１．以雌蕊组织作外植体时,仅附加外源细胞分裂素就可以诱导果实状结构的再生,外源生长素似乎不是必需的,最高的诱导频率（５０．０％ ）出现在仅附加玉米素０．５ ｍ ｇ／Ｌ的组合。２．从直径４—１２ ｍ ｍ 的幼果上分离的外植体在附加外源激素的培养基上均可诱导果实状结构的再生,但只有从直径８ ｍ ｍ 的果实分离的组织块作外植体并将它们培养在６－ＢＡＰ ２ ｍ ｇ／Ｌ,ＮＡＡ０．１ ｍ ｇ／Ｌ的培养基上时,果实状结构的诱导频率最高（６２．５％ ）。为了探讨在果实状结构再生中表现出来的细胞全能性的表达,提出了植物细胞全能性的部分表达（Ｐａｒｔｉａｌｅｘｐｒｅｓｓｉｏｎ ｏｆｐｌａｎｔ ｃｅｌｌｔｏｔｉｐｏｔｅｎｃｙ）的概念并进行了讨论。     

灵芝免疫调节蛋白(Lz-8)在毕赤酵母中的表达及其免疫活性鉴定

真菌免疫调节蛋白家族(Fungi immunoregulatory proteins,FIPs)各成员所具有的免疫调节和抗肿瘤活性已被广泛研究。本研究利用毕赤酵母表达系统对其成员Lz-8进行了重组表达。以毕赤酵母突变株GS115为表达宿主细胞,PCR和DNA测序结果均显示Lz-8的cDNA已被成功地整合入酵母基因组。聚丙烯酰胺凝胶电泳(SDS-PAGE)、激光解析飞行时间质谱(MALDI-TOF-MS)和免疫学实验均被用于重组表达蛋白的检测。实验结果表明Lz-8在毕赤酵母表达系统中得到成功表达,在SDS-PAGE中可观察到分子量为14000D的单一条带,MALDI-TOF-MS的实验结果显示rLz-8的分子量为12722D。在相关的免疫学实验中,rLz-8可引起绵羊血红细胞凝集,但对人血4种血型的红细胞并没有凝集作用,rlz-8还可诱导巨噬细胞吞噬作用,均与其他报道中的实验结果吻合。以上结果表明,本实验已成功地利用毕赤酵母表达系统对Lz-8进行重组表达。     

Elevated intracellular cyclic-di-GMP level in Shewanella oneidensis increases expression of c-type cytochromes

Electrochemically active biofilms are capable of exchanging electrons with solid electron acceptors and have many energy and environmental applications such as bioelectricity generation and environmental remediation. The performance of electrochemically active biofilms is usually dependent on c-type cytochromes, while biofilm development is controlled by a signal cascade mediated by the intracellular secondary messenger bis-(3ʹ-5ʹ) cyclic dimeric guanosine monophosphate (c-di-GMP). However, it is unclear whether there are any links between the c-di-GMP regulatory system and the expression of c-type cytochromes. In this study, we constructed a S. oneidensis MR-1 strain with a higher cytoplasmic c-di-GMP level by constitutively expressing a c-di-GMP synthase and it exhibited expected c-di-GMP-influenced traits, such as lowered motility and increased biofilm formation. Compared to MR-1 wild-type strain, the high c-di-GMP strain had a higher Fe(III) reduction rate (21.58 vs 11.88 pM of Fe(III)/h cell) and greater expression of genes that code for the proteins involved in the Mtr pathway, including CymA, MtrA, MtrB, MtrC and OmcA. Furthermore, single-cell Raman microspectroscopy (SCRM) revealed a great increase of c-type cytochromes in the high c-di-GMP strain as compared to MR-1 wild-type strain. Our results reveal for the first time that the c-di-GMP regulation system indirectly or directly positively regulates the expression of cytochromes involved in the extracellular electron transport (EET) in S. oneidensis, which would help to understand the regulatory mechanism of c-di-GMP on electricity production in bacteria.