七姊妹山常绿落叶阔叶混交林物种多样性格局及其环境解释

依托七姊妹山自然保护区6 hm²森林动态监测样地研究平台,基于样地和物种基本信息数据,采用多元回归树和冗余分析研究方法,探讨地形因子对生境的塑造作用及物种分布特征,分析不同群丛类型下物种多样性的变化规律。结果表明：(1)依据“1 SE”规则,4次分割依次以海拔(1 453 m)、坡度(23.13°)、海拔(1 398 m)、凹凸度(4.094)为分界点可将150个样地分为5个群丛。(2)冗余分析表明地形因子对物种分布解释量为0.077 6,解释率为16.36%,各环境因子对物种分布的解释力度依次为：海拔>坡度>凹凸度;坡向与物种的分布无显著相关性。(3)5个群丛中立木密度与胸高截面积最高的均为群丛5(527.4株/400 m²;3.495 cm²/株),立木密度与平均胸高截面积最低为群丛4(225.4株/400 m²;3.057 cm²/株)。(4)5个群丛中Shannon Winener丰富度指数与Simpson优势度指数最高的均为群丛2,最低的为群丛5,物种多样性尺度效应明显;Pielou均匀度指数最高为群丛4,最低为群丛5。(5)两两群丛间Jaccard相似性系数最低为群丛1 群丛2(0.331),最高的为群丛4 群丛5(0.645),海拔对β多样性格局影响较大。研究认为,七姊妹山自然保护区6 hm²样地地形因子对该区域生境的塑造具有一定作用,海拔、坡度、凹凸度组成的“环境筛”影响了该区域的物种分布及多样性格局。     

前列腺癌细胞来源的外泌体诱导巨噬细胞极化

外泌体(exosome)是直径约30～150 nm的由细胞分泌的一种具有生物学活性的囊泡。有些来自癌细胞的外泌体可以将巨噬细胞(macrophages,Mφ)极化为M2亚型,但前列腺癌细胞来源的外泌体在巨噬细胞极化中的作用仍缺乏研究。本研究采用超滤法提取前列腺癌细胞PC-3M-2B4和PC-3M-IE8条件培养基中的外泌体(PCa-exo)。分别用透射电子显微镜、纳米粒径分析及Western印迹对外泌体形态、颗粒大小和表面的特异性分子标志进行分析鉴定。用PKH67标记外泌体,观察PCa-exo能否被巨噬细胞吸收。免疫荧光分析PCa-exo处理巨噬细胞后,M2型巨噬细胞表面分子标志CD206的表达差异。用q-PCR观察PCa-exo诱导后的巨噬细胞中IL-10、IL-1β等细胞因子的表达。电镜、Western印迹和纳米粒径分析的结果显示,PCa-exo形态多为圆形,直径约为40～150 nm,PCa-exo能被巨噬细胞大量吸收。PCa-exo诱导后,巨噬细胞中CD206荧光表达显著增高,IL-10、IL-1β及IL-12等炎症因子的表达水平与M2/TAM亚型巨噬细胞的表达谱一致。本研究表明,前列腺癌细胞来源的外泌体能诱导巨噬细胞极化为M2表型。     

蔓茎堇菜和柔毛堇菜多糖的抑菌抗氧化活性

利用乙醇沉淀法提取蔓茎堇菜Viola diffusa和柔毛堇菜V.principis多糖并分别进行抑菌及抗氧化试验。结果表明,蔓茎堇菜和柔毛堇菜多糖提取率分别为7.0%和8.3%。不同倍数体积无水乙醇沉淀提取的多糖抑菌和抗氧化能力不同。抑菌效果显示,蔓茎堇菜多糖对大肠杆菌和枯草芽孢杆菌的抑菌圈分别可达8.46mm和8.59mm,柔毛堇菜对大肠杆菌和枯草芽孢杆菌的抑菌圈均可达9.13mm,但两种堇菜多糖对黑曲霉和啤酒酵母未呈现抑制活性;抗氧化研究发现,蔓茎堇菜多糖抗氧化活性为243.64U·mL^-1,柔毛堇菜多糖抗氧化活性为411.78U·mL^-1。由此可见,无论是抑菌还是抗氧化活性方面,柔毛堇菜极显著优于蔓茎堇菜(P<0.01)。蔓茎堇菜和柔毛堇菜多糖都具有一定的抑菌抗氧化活性,均可作为食药两用植物资源进行开发利用。     

新型2-喹诺酮类Polo样激酶1抑制剂的设计合成及分子对接研究

目的:设计合成新型2-喹诺酮类Polo样激酶1(Plk1)抑制剂。方法:以Plk1抑制剂ON 01910为先导化合物,利用生物电子等排原理设计一系列2-喹诺酮类衍生物,用Autodock软件将该类化合物与Plk1进行分子对接和虚拟筛选,计算结合自由能;以取代的氯(溴)苄为起始原料,先后经巯基乙酸取代、双氧水氧化、与(对甲氧基)苯胺酰化,再经环合、水解制得目标化合物。结果:设计的化合物大多数与Plk1的结合自由能均比ON 01910的低,结合强度高、稳定性好;合成了16个2-喹诺酮类衍生物,产物结构经1H-NMR确证。结论:所得化合物中有15个为新化合物,化合物的结构设计科学合理,虚拟筛选结果良好,为后续实体筛选和化合物结构优化提供了理论依据和参考。     

莼菜休眠芽解除休眠及生根的研究

莼菜为世界著名珍稀水生蔬菜,具有很高的食用和药用价值。已有研究显示,可通过冬芽实现莼菜复壮,找出休眠解除的最佳方法是复壮的基本前提。本实验以莼菜冬季型休眠芽（冬芽）为实验材料,通过光照、温度等处理探求莼菜冬芽的休眠解除方法。莼菜冬芽生根率随着光照强度的增加,其生根率由全黑暗0%显著增长至（16.0±1.3）%;温度和处理时间对莼菜冬芽生根率、根长、生根根数和含水量有显著性影响。其中,35 °C水浴处理6 h后各项指标均到达较大值,上述指标分别为（96.1±2.8）%、（7.2±0.2） cm、74.5±6.0和（83.6±0.3）%;40 °C（6 h）、45 °C（1、3和6 h）和50 °C（10、20和30 min）水浴处理后莼菜冬芽绝大部分失绿变黄;随着培养时间的延长,其冬芽全部腐烂。光照能够促进莼菜冬芽生根;土培生根效果较为显著;适度水浴加热处理能有效解除莼菜冬芽的休眠,35 °C水浴处理6 h为最佳处理方案。     

适合免疫治疗的大鼠抗肾小球基底膜肾炎模型的建立

以线性表位肽P14（a3_127-148）作为抗原建立适合免疫治疗的抗肾小球基底膜（anti-glomerular basement membrane,GBM）病大鼠模型。采用大鼠后脚垫三点注射P14（a3_127-148）与弗氏佐剂乳化物的方法进行单次免疫,免疫前后每周采集24 h尿样和血样,所有大鼠在免疫后7 w处死。大鼠免疫后,肾炎模型组在各时间点的24 h尿蛋白、尿蛋白肌酐比值（albumin/urine creatinine ratio,ACR）、血肌酐及血尿素氮均明显高于对照组（P<0.05）;循环抗P14（a3_127-148）IgG抗体水平明显高于对照组(P<0.001);PAS染色可见节段性纤维素样坏死,富于细胞型新月体;免疫组化染色可见肾小球有明显的中性粒细胞和巨噬细胞浸润;免疫荧光检测可见IgG沿GBM呈强线性沉积;电镜观察到GBM的断裂和收缩;而对照组均未见改变。HE染色在所有大鼠中均未观察到肺部病变。使用P14（a3_127-148）线性肽免疫WKY大鼠成功建立了大鼠抗GBM病模型,有助于开发更为特异的免疫疗法。     

hPEBP4 resists TRAIL-induced apoptosis of human prostate cancer cells by activating Akt and deactivating ERK1/2 pathways

The treatment options available for prostate cancer are limited because of its resistance to therapeutic agents. Thus, a better understanding of the underlying mechanisms of the resistance of prostate cancer will facilitate the discovery of more efficient treatment protocols. Human phosphatidylethanolamine-binding protein 4 (hPEBP4) is recently identified by us as an anti-apoptotic molecule and a potential candidate target for breast cancer treatment. Here we found the expression levels of hPEBP4 were positively correlated with the severity of clinical prostate cancer. Furthermore, hPEBP4 was not expressed in TRAIL-sensitive DU145 prostate cancer cells, but was highly expressed in TRAIL-resistant LNCaP cells, which show highly activated Akt. Interestingly, hPEBP4 overexpression in TRAIL-sensitive DU145 cells promoted Akt activation but inhibited ERK1/2 activation. The hPEBP4-overexpressing DU145 cells became resistant to TRAIL-induced apoptosis consequently, which could be reversed by PI3K inhibitors. In contrast, silencing of hPEBP4 in TRAIL-resistant LNCaP cells inhibited Akt activation but increased ERK1/2 activation, resulting in their sensitivity to TRAIL-induced apoptosis that was restored by the MEK1 inhibitor. Therefore, hPEBP4 expression in prostate cancer can activate Akt and deactivate ERK1/2 signaling, leading to TRAIL resistance. We also demonstrated that hPEBP4-mediated resistance to TRAIL-induced apoptosis occurred downstream of caspase-8 and at the level of BID cleavage via the regulation of Akt and ERK pathways, and that hPEBP4-regulated ERK deactivation was upstream of Akt activation in prostate cancer cells. Considering that hPEBP4 confers cellular resistance to TRAIL-induced apoptosis and is abundantly expressed in poorly differentiated prostate cancer, silencing of hPEBP4 suggests a promising approach for prostate cancer treatment.     

Effect of Human WEE1 and Stem Cell Factor on Human CD34^＋ Umbilical Cord Blood Cell Damage Induced by Chemotherapeutic Agents

Myelosuppression is one of the major side-effects of most anticancer drugs. To achieve myeloprotection, one bicistronic vector encoding anti-apoptotic protein human WEE l （WEElHu） and proliferation-stimulating stem cell factor （SCF） was generated. In this study, we selected human umbilical cord blood CD34^＋ cells as the in vitro model in an attempt to investigate whether WEEIHu, rather than conventional drug-resistant genes, can be introduced to rescue cells from the damage by chemotherapeutic agents such as cisplatin, adriamycin, mitomycin-c and 5-fluorouracil. Cell viability and cytotoxicity assay, colony-forming units in culture assay and externalization of phospholipid phosphatidylserine analysis showed that the expression of WEElHu and SCF in CD34^＋ cells provided the cells with some protection. These findings suggest that the expression of WEElHu and SCF might rescue CD34^＋ cells from chemotherapyinduced myelosuppression.     

粉背含笑，云南东南部木兰科植物一新种

本新种与皱皮杜鹃(Rhododendron wiltonii Hemsl.et Wils.)相近似,区别在于前者叶较小,长6.8～8.0 cm,宽2.0～2.5 cm,叶表面平坦而不呈泡状突起,叶背密被一层黄色至锈红色毡毛,花5～6（～9）朵,较小,长约2.5 cm,易于区别。     

蒙古沙鼠脑缺血后大脑皮质Calretinin(CR)的表达变化

目的:观察蒙古沙鼠前脑短暂缺血后前额皮质Calretinin(CR)的表达变化,为进一步研究其功能及治疗提供形态学依据。方法:24只健康雄性长爪鼠随机分为正常组对照组(6只)和缺血组(18只),夹闭蒙古沙鼠双测颈总动脉10 min诱导前脑缺血后,动物分别存活1天、3天或7天。用免疫组织化学方法检测了前额皮质中CR的表达。结果:与正常组相比,各缺血组中前额皮质中CR表达均上调。缺血再灌1天时,CR表达最强(P＜0．01);3天时CR表达开始恢复(P＜0．05);7天时CR表达进一步恢复,但仍高于正常组(P＜0．01)。结论:前脑短暂缺血后可造成蒙古沙鼠前额皮质CR的表达在短时间内急剧上调;但随着时间的CR的表达会恢复正常。