油脂废水生物处理研究进展

目前,油脂降解在常规的废水生物处理工艺中没有得到充分重视,造成反应器的处理效率大大降低,因此成熟有效的油脂降解生物处理技术开发与应用有待于深入探讨.本文系统阐述了废水处理过程中油脂的生物降解途径与机理,重点总结了油脂降解途径中油脂水解与长链脂肪酸降解涉及的功能微生物研究等最新进展,简要介绍了部分学者根据功能微生物的生境差别开发的一系列新型处理工艺,并在此基础上展望了油脂降解技术研究的重点突破方向,希望能为该工艺的发展提供理论指导.     

氧化还原对成年大鼠海马CA1区锥体神经元外向整流氯通道的调控作用

采用膜片钳内面向外式记录技术,研究急性分离成年大鼠海马CAl区锥体神经元外向整流氯离子通道的氧化还原调控。发现细胞内侧给予氧化剂DTNB(5,5'-dithiobis-2-nitrobenzoic acid),可显著减弱氯通道的活动,IC50值为(28.05±2.42)μmol/L;还原剂DTT(dithiothreitol)对氯通道没有明显影响,但可逆转DTNB引起的抑制效应。说明DTNB不改变通道电导,其引起的通道活动减弱是由氯通道关闭时间延长而开放时间缩短所致。研究还发现,另一对氧化型和还原型谷胱甘肽具有与DTNB和DTT同样的效应。本研究结果显示,成年大鼠海马CA1区锥体神经元外向整流氯通道可以被细胞内氧化还原剂所调控。     

c-src在大鼠卵巢中的表达及其在原始卵泡生长启动中的作用初探

目的：研究原癌基因c-src在大鼠卵巢的表达,及其在原始卵泡启动过程中的作用。方法：取2日龄SD雌性大鼠卵巢,在Waymouth培养体系中培养0．4、8d后,首先采用RT-PCR方法证实大鼠卵巢中有c-src的表达,再体外合成其RNA小干扰片段（small interference RNA,siRNA）转染培养中的卵巢组织进行RNA干扰,用HE染色及RT-PCR筛选最佳干扰片断并用慢病毒包装后检测干扰效果。结果：随着培养天数的增加,原始卵泡在卵泡总数中所占比例逐渐减少;c—src mRNA在原始卵泡中有表达,经筛选用最佳干扰片断siRNA1慢病毒包装进行RNA干扰,发现干扰后,与空白组、空白载体组相比,最佳干扰组c—src mRNA含量明显下降,原始卵泡在卵泡总数中所占比例相对更多,原始卵泡发育受到抑制。结论：c-src在原始卵泡中有表达,并在一定程度上促进了原始卵泡的发育。     

低氧脑水肿大鼠脑组织VEGF和AQPs基因及蛋白表达的变化

目的：探讨低氧脑水肿时血管内皮细胞生长因子（VEGF）、水通道蛋白（AQP1和AQP4）基因和蛋白表达变化,为阐明急性低氧对脑组织的损伤及低氧脑水肿的发病机制提供实验依据。方法：Wistar大鼠随机分为4个组：常氧对照组（Control）、低氧暴露4 000 m组（4 000 m）、低氧暴露6 000 m组（6 000 m）和低氧暴露8 000 m组（8 000 m）,低氧组于低压舱中模拟相应海拔高度持续暴露8 h建立低氧脑水肿模型。用干-湿重法测定脑组织水含量,常规光镜观察脑组织形态学的改变;用RT-PCR法和免疫组化法检测低氧脑水肿时大鼠脑组织VEGF、AQP1和AQP4mRNA和蛋白表达的变化。结果：①干-湿重法测定表明,低氧（≥6 000 m）暴露后,大鼠脑组织水含量明显增加（P〈0.01）。②常规光镜检测结果表明,低氧暴露4 000 m时大鼠脑神经细胞、血管内皮细胞和星形胶质细胞足突轻度肿胀,组织中出现漏出液;低氧暴露6 000 m时脑血管内皮细胞和星形胶质细胞足突肿胀加重,血管与组织间隙扩大,组织中漏出液增多;低氧暴露8 000m时脑血管内皮细胞和星形胶质细胞足突重度肿胀,血管与组织间隙进一步扩大,组织中漏出液明显增多。③低氧脑水肿时,VEGF、AQP1、AQP4mRNA表达水平增高,AQP1在内皮细胞异常表达,内皮细胞VEGF和AQP1、星形胶质细胞足突AQP4蛋白质表达水平增高。结论：低氧脑水肿时,VEGF、AQP1和AQP4表达和分布的变化可能是引起血脑屏障损伤、导致低氧脑水肿的发病机制之一。     

Effects of land use pattern on soil microbial biomass carbon in Xishuangbanna

In January 2006 - September 2007, a controlled litter-removal and root-cutting experiment was conducted to study the effects of different land use patterns (secondary forest or rubber plantation) on soil microbial biomass carbon in Xishuangbanna, China. After the secondary forest converted into rubber plantation, soil nutrient contents and plant carbon input decreased obviously, and soil microbial biomass carbon had a significant decrease. These two forest types had a higher soil microbial biomass carbon in rainy season than in dry season. In secondary forest, soil microbial biomass carbon was significantly positively correlated with soil temperature; while in rubber plantation, the microbial biomass carbon was positively correlated with soil moisture. In secondary forest, soil microbial biomass carbon was controlled by the nutrient inputs from plant roots, but less affected by litter amount. Also in secondary forest, soil microbial biomass carbon was significantly positively correlated with fine-root biomass and its C and N inputs. In rubber plantation, both the fine-root biomass and its C and N inputs and the litter amount had lesser effects on soil microbial biomass carbon. These results suggested that planting rubber induced the decreases of soil nutrient contents and pH value, and, added with serious artificial disturbances, reduced the soil microbial biomass carbon and changed its controlling factors, which in turn would affect other soil ecological processes.     

泰山沙参属植物资源调查与营养成分分析

目的:了解泰山沙参属植物资源现状,测定其根中脂肪、蛋白质及多糖的含量,为合理开发利用泰山沙参属植物资源提供依据。方法:采用野外实地调查法进行资源考察;分别用索氏提取法、考马斯亮蓝法和苯酚-硫酸法测定脂肪、蛋白质和多糖的含量。结果:采集的100余份标本,经鉴定为沙参属植物狭叶沙参[Adenophora gmeli-nii(Spreng)Fisch.]、石沙参(Adenophora polyantha Nakai)、杏叶沙参(Adenophora stricta Mig.)及细叶沙参(Adeno-phora paniculata Nannf.)。泰山沙参属植物狭叶沙参、石沙参、杏叶沙参和细叶沙参脂肪含量分别为2.14%～7.34%,4.27%～7.72%1,.54%～2.51%和4.98%。蛋白质含量分别为0.60～2.10 mg/g0,.80～1.89 mg/g,0.83～0.89 mg/g和1.05 mg/g,多糖含量分别为20.58%～63.21%2,7.74%～65.14%,43.14%～48.47%和45.60%。结论:泰山野生沙参属植物资源丰富,品种多、分布广、蕴藏量大,多糖含量较高,具有较大的开发前景。     

Identification of QTLs for seed germination capability after various storage periods using two RIL populations in rice

Seed germination capability of rice is one of the important traits in the production and storage of seeds. Quantitative trait loci (QTL) associated with seed germination capability in various storage periods was identified using two sets of recombinant inbred lines (RILs) which derived from crosses between Milyang 23 and Tong 88-7 (MT-RILs) and between Dasanbyeo and TR22183 (DT-RILs). A total of five and three main additive effects (QTLs) associated with seed germination capability were identified in MT-RILs and DT-RILs, respectively. Among them, six QTLs were identified repeatedly in various seed storage periods designated as qMT-SGC5.1, qMT-SGC7.2, and qMT-SGC9.1 on chromosomes 5, 7, and 9 in MT-RILs, and qDT-SGC2.1, qDT-SGC3.1, and qDT-SGC9.1 on chromosomes 2, 3, and 9 in DT-RILs, respectively. The QTL on chromosome 9 was identified in both RIL populations under all three storage periods, explaining up to 40% of the phenotypic variation. Eight and eighteen pairs additive × additive epistatic effect (epistatic QTL) were identified in MT-RILs and DT-RILs, respectively. In addition, several near isogenic lines (NILs) were developed to confirm six repeatable QTL effects using controlled deterioration test (CDT). The identified QTLs will be further studied to elucidate the mechanisms controlling seed germination capability, which have important implications for long-term seed storage.     

Assembly mechanism of [Fe2S2] cluster in ferredoxin from Acidithiobacillus ferrooxidans

Ferredoxin is a typical iron-sulfur protein that is ubiquitous in biological redox systems. This study investigates the in vitro assembly of a [Fe2S2] cluster in the ferredoxin from Acidithiobacillus ferrooxidans in the presence of three scaffold proteins: IscA, IscS, and IscU. The spectra and MALDI-TOF MS results for the reconstituted ferredoxin confirm that the iron-sulfur cluster was correctly assembled in the protein. The inactivation of cysteine desulfurase by L-allylglycine completely blocked any [Fe2S2] cluster assembly in the ferredoxin in E. coli, confirming that cysteine desulfurase is an essential component for iron-sulfur cluster assembly. The present results also provide strong evidence that [Fe2S2] cluster assembly in ferredoxin follows the AUS pathway.     

Development of a quantitative PCR for detection of Lactobacillus plantarum starters during wine malolactic fermentation

A quantitative, real-time PCR method was developed to enumerate Lactobacillus plantarum IWBT B 188 during the malolactic fermentation (MLF) in Grauburgunder wine. The qRT-PCR was strain-specific, as it was based on primers targeting a plasmid DNA sequence, or it was L. plantarum-specific, as it targeted a chromosomally located plantaricin gene sequence. Two 50 l wine fermentations were prepared. One was inoculated with 15 g/hl Saccharomyces cerevisiae, followed by L. plantarum IWBT B 188 at 3.6 × 10(6) CFU/ml, whereas the other was not inoculated (control). Viable cell counts were performed for up to 25 days on MRS agar, and the same cells were enumerated by qRT-PCR with both the plasmid or chromosomally encoded gene primers. The L. plantarum strain survived under the harsh conditions in the wine fermentation at levels above 10(5)/ml for approx. 10 days, after which cell numbers decreased to levels of 10(3) CFU/ml at day 25, and to below the detection limit after day 25. In the control, no lactic acid bacteria could be detected throughout the fermentation, with the exception of two sampling points where ca. 1 × 10(2) CFU/ml was detected. The minimum detection level for quantitative PCR in this study was 1 × 10(2) to 1 × 10(3) CFU/ml. The qRT-PCR results determined generally overestimated the plate count results by about 1 log unit, probably as a result of the presence of DNA from dead cells. Overall, qRT-PCR appeared to be well suited for specifically enumerating Lactobacillus plantarum starter cultures in the MLF in wine.     

Sepiapterin improves angiogenesis of pulmonary artery endothelial cells with in utero pulmonary hypertension by recoupling endothelial nitric oxide synthase

Persistent pulmonary hypertension of the newborn (PPHN) is associated with decreased blood vessel density that contributes to increased pulmonary vascular resistance. Previous studies showed that uncoupled endothelial nitric oxide (NO) synthase (eNOS) activity and increased NADPH oxidase activity resulted in marked decreases in NO bioavailability and impaired angiogenesis in PPHN. In the present study, we hypothesize that loss of tetrahydrobiopterin (BH4), a critical cofactor for eNOS, induces uncoupled eNOS activity and impairs angiogenesis in PPHN. Pulmonary artery endothelial cells (PAEC) isolated from fetal lambs with PPHN (HTFL-PAEC) or control lambs (NFL-PAEC) were used to investigate the cellular mechanisms impairing angiogenesis in PPHN. Cellular mechanisms were examined with respect to BH4 levels, GTP-cyclohydrolase-1 (GCH-1) expression, eNOS dimer formation, and eNOS-heat shock protein 90 (hsp90) interactions under basal conditions and after sepiapterin (Sep) supplementation. Cellular levels of BH4, GCH-1 expression, and eNOS dimer formation were decreased in HTFL-PAEC compared with NFL-PAEC. Sep supplementation decreased apoptosis and increased in vitro angiogenesis in HTFL-PAEC and ex vivo pulmonary artery sprouting angiogenesis. Sep also increased cellular BH4 content, NO production, eNOS dimer formation, and eNOS-hsp90 association and decreased the superoxide formation in HTFL-PAEC. These data demonstrate that Sep improves NO production and angiogenic potential of HTFL-PAEC by recoupling eNOS activity. Increasing BH4 levels via Sep supplementation may be an important therapy for improving eNOS function and restoring angiogenesis in PPHN.