内循环颗粒污泥床硝化反应器流动模型研究

采用脉冲刺激响应技术,对稳态内循环颗粒污泥床硝化反应器进行了示踪试验。根据试验结果,分别运用轴向扩散模型和多釜全混流反应器串联模型,对反应器沉淀区和循环区的流态进行了分析和判断。结果表明,反应器沉淀区的分散数D/uL为0.00148,该区域的流态接近于平推流反应器（PFR）;反应器循环区的串联级数为1.021,该区域的流态接近于全混流反应器（CSTR）。稳态时,反应器的理论水力停留时间为360min,实际水力停留时间为341.2min,反应器中死区所占的体积百分比为5.22％,其中生物体死区为0.75%,水力死区为4.47%,表明反应器结构性能良好。根据试验和分析结果,建立了内循环颗粒污泥床硝化反应器的流动模型,即全混流和平推流的串联组合模型。由流动模型所得的理论停留时间分布曲线与由试验所得的实际停留时间分布曲线吻合良好,两者的平均相对误差为8.56%,表明所建模型具有较高的准确性。     

食物在贻贝棘尾虫(原生动物,纤毛虫)细胞内的消化过程

利用免疫荧光显微术、透射电镜及电镜酶细胞化学技术对食物在腹毛类纤毛虫-- 贻贝棘尾虫细胞内的消化过程进行了追踪观察.食物在进入消化腔隙的初期,外面包被着一层膜结构,但此外层膜很快被消化而消失;尔后食物在贻贝棘尾虫体内的消化过程可分为两种方式:一种方式为直接在消化腔隙内完成,此过程同1982年Kaul et al.和Das s et al.的报道;而另一部分食物的消化过程表现为食物逐步向细胞质内突入,以致最终完全被细胞质包围形成一被膜包裹的圆泡状结构;在此过程中,细胞质边缘突出众多含有酸性磷酸酶等物质的小囊泡结构,小囊泡与食物融合,其内的酸性磷酸酶等水解酶释放出来, 食物的表膜逐渐瓦解,个体逐渐变小,最终消化后的营养物质被释放到细胞的消化腔隙内; 这种食物通过胞口与胞咽达消化腔隙后,再由细胞质将其包裹形成的食物泡,我们称之为" 后成食物泡".这两种消化方式与贻贝棘尾虫的消化胞器为一腔隙结构相适应[动物学报 5 4(3):510-516,2008].     

用间接免疫荧光法检测流行性出血热病人尿中特异性抗体的研究

用间接免疫荧光法检测110例不同病程、病期及病型的流行性出血热病人尿中及血清中特异性抗体。尿中IgM型抗体阳性率为62.7％。尿中IgG型抗体阳性率91.8％与血清IgG型者90.9％相似,而总阳性率(IgG或IgM有一项以上阳性者的总检出率)99.1％则高于血清IgG者。20例其它疾病及10例正常人尿抗体均为阴性。结果表明尿抗体检查法是特异且可靠的,它比血清学方法简便、灵敏、为临床诊断可早期快速得出结果,不用采血有利于病人。IgM型抗体阳性率受病程、病期、病型及尿蛋白量的影响较明显。     

简单快速的植物花粉母细胞分裂期染色体致畸研究的制片技术

本文描述了改进的简单、快捷、效果好的植物花粉母细胞分裂时期染色体致畸研究的制片技术程序,及其在环境生物研究中的重要意义。它比其它技术节省时间达24～30小时。     

昆虫种群的遗传调控

昆虫种群的遗传调控是利用昆虫自身生长发育的关键基因,采用性别控制开关,通过遗传转化使雄虫成为携带导致后代雌虫发育异常或雌性不育的遗传控制复合体（性别开关元件和靶标基因的复合体）．昆虫种群遗传调控是一种基于不育技术的昆虫种群控制系统,具有种类特异、环境友好和便捷高效等特点．目前为止,已经由早期的通过辐射不育方法发展到释放携带显性致死基因昆虫的方法,并在多种昆虫中获得成功．本文综述了昆虫种群遗传调控的发展历程,介绍了昆虫种群遗传调控相关的理论与方法,包括特异的调控元件、致死或缺陷基因和遗传转化体系的应用,并列举了几种昆虫种群遗传调控的实例,最后对于昆虫种群遗传调控系统中存在的问题以及可能的发展方向进行了展望．     

Microstructures formed in aqueous solutions of a hydrophobically modified nonionic cellulose derivative and sodium dodecyl sulfate: a fluorescence probe investigation

The association behavior of hydrophobically modified ethyl hydroxyethyl cellulose (HM-EHEC) and its interaction with the anionic surfactant sodium dodecyl sulfate (SDS) has been studied in the dilute concentration regime. Steady-state fluorescence probe techniques have been utilized to obtain microstructural information of the system properties and combined with macroscopic bulk information from equilibrium dialysis experiments in order to determine binding isotherms of SDS to HM-EHEC. HM-EHEC was found to self-associate and form polymeric micelles in semi-dilute aqueous solutions. c^* for the self-association process was determined to be approximately 0.4%. The microviscosity of the polymeric micelles is much higher, and the micropolarity slightly higher, than that of ordinary SDS micelles. The onset of interaction between HM-EHEC and SDS was evidenced by a simultaneous strong increase in microviscosity and decrease in micropolarity upon successive addition of SDS. There is a minor, noncooperative SDS binding to the HM-EHEC starting from low concentrations of SDS (<5 mM) followed by a highly cooperative binding region at SDS concentrations ≥5 mM. The polymer–surfactant aggregates are rigid and hydrophobic with a maximum in microviscosity in the noncooperative binding region at a very low degree of SDS-adsorption.     

Using RNA-mediated Interference Feeding Strategy to Screen for Genes Involved in Body Size Regulation in the Nematode C. elegans

Double-strand RNA-mediated interference (RNAi) is an effective strategy to knock down target gene expression^1-3. It has been applied to many model systems including plants, invertebrates and vertebrates. There are various methods to achieve RNAi in vivo^4,5. For example, the target gene may be transformed into an RNAi vector, and then either permanently or transiently transformed into cell lines or primary cells to achieve gene knockdown effects; alternatively synthesized double-strand oligonucleotides from specific target genes (RNAi oligos) may be transiently transformed into cell lines or primary cells to silence target genes; or synthesized double-strand RNA molecules may be microinjected into an organism. Since the nematode C. elegans uses bacteria as a food source, feeding the animals with bacteria expressing double-strand RNA against target genes provides a viable strategy⁶. Here we present an RNAi feeding method to score body size phenotype. Body size in C. elegans is regulated primarily by the TGF- β - like ligand DBL-1, so this assay is appropriate for identification of TGF-β signaling components⁷. We used different strains including two RNAi hypersensitive strains to repeat the RNAi feeding experiments. Our results showed that rrf-3 strain gave us the best expected RNAi phenotype. The method is easy to perform, reproducible, and easily quantified. Furthermore, our protocol minimizes the use of specialized equipment, so it is suitable for smaller laboratories or those at predominantly undergraduate institutions.     

果树盲蝽的发生与防控技术

近年来,盲蝽在我国果树上大量发生,刺吸危害枣、葡萄、苹果、梨、樱桃、桃树等果树,造成嫩芽皱缩,落蕾落花,叶片穿孔,水果畸形脱落,导致严重的经济损失。本文介绍了我国果树上盲蝽的种类、危害和发生规律,综述了果树盲蝽防治策略和防治措施,提出了果树盲蝽的防控对策和建议。     

宫颈特殊染色技术对子宫颈癌及宫颈上皮内瘤变初筛的临床研究

目的:探讨宫颈特殊染色技术筛查方法对宫颈癌及癌前病变的筛查意义。方法:本研究通过对1963例就诊我院妇科门诊的患者进行宫颈特殊染色检查(FRD),以组织病理学检查结果为标准,分析FRD宫颈特殊染色的临床意义。结果:1963例患者行宫颈特殊染色检查及对初筛阳性患者行阴道镜下活检,根据活检病理结果进行分析,CINI阳性率80.77%℅,CINII81.25%,CINIII100%℅,侵润癌100%,总阳性率90.50%。结论:利用亚甲蓝显色和醋酸白化反应双重定位及指示,不仅可提高宫颈癌及癌前病变的检出率,而且操作简便,判读容易,结果快速,成本低廉。     

百合生殖细胞分裂过程中微管分布的显微荧光观察

用抗微管蛋白抗体和荧光标记技术,观察了百合生殖细胞经有丝分裂形成精细胞过程中微管的变化。生殖细胞在分裂的前期,存在于核外围以及细胞两端胞质内的微管大都以微管束的形式沿细胞长轴方向平行排列。在靠近核的部位,有些微管有时会斜向排列。分裂进入中期后,染色体集中排列在赤道面。在染色体周围可以见到有多束与细胞长轴平行排列着的微管,但这些微管束是在分裂中期时新形成的或是在前期已存在,尚难以断定。这些微管束有一个特点,就是当它们延伸至赤道板部位时,在每一条微管束上都有一个无荧光的小圆区;这个小圆区可能代表着丝粒的位置。细胞分裂进入后期,姊妹染色单体分别向两极移动形成两组染色体。在它们之间近赤道板位置出现了一个具有强烈荧光的区域,显示在这一部位,微管相当浓密。从这一强烈荧光区向两极分别伸出多条微管束。因此,在这一强烈荧光区内可能有多个微管束重叠。到细胞分裂末期,在这一强烈的荧光区的中央出现了一条横向的无荧光区。这一区域有可能为胞质完成分裂后新形成的细胞板所在的部位。