濒危植物金花猕猴桃繁殖生物学初步研究

繁殖生物学是目前濒危植物保护生物学研究的重点领域之一,金花猕猴桃(Actinidia chrysantha)是猕猴桃属濒危物种之一,目前未见其繁殖生物学相关报道。因此,该文以分布于花坪国家级自然保护区的野生金花猕猴桃为研究对象,用游标卡尺测量了花器官及果实形态,通过野外观察记录了其物候、访花昆虫及开花结果习性,用人工授粉和套袋法确定其传粉媒介,开展田间播种试验确定种子繁殖力,对其繁殖生物学开展了较为系统的研究。结果表明：金花猕猴桃物候因海拔高度不同而不同,较低海拔地区5月中下旬开花,高海拔地区5月下旬至6月上旬开花,花期持续7~10 d,果实每年9月下旬至10月上旬成熟;雄株花枝率76.5％,雌株果枝率61.9％,果实长圆柱形、短圆柱形或椭圆形,平均单果重7.34~27.53 g,最大果重35.0 g;金花猕猴桃为虫媒和风媒共同授粉,主要访花昆虫有蜜蜂科、细蜂科、鼻蝇亚科、食蚜蝇科、蜡蝉科、大蚊科长脚蚊属昆虫等;金花猕猴桃种子发芽率低,参试的3个居群的种子发芽率存在差异,分别为花坪17.5％,资源车田15.36％,贺州姑婆山0;4种不同种子处理方式中,低温＋GA3处理的种子发芽率(22.67％)最高。综上所述,金花猕猴桃不存在传粉障碍,种子萌发率低可能是致其濒危的重要原因。该研究结果为保护金花猕猴桃种质资源提供了科学依据。     

巴氏蘑菇子实体不同发育阶段的转录组分析

为探讨巴氏蘑菇子实体不同发育阶段基因的表达情况,本研究对巴氏蘑菇子实体不同发育时期（原基、采收期和开伞期）进行转录组测序,以本实验室已获得的巴氏蘑菇JA菌株的不育单孢菌株JA-15036基因组为参考基因组研究原基与采收期及开伞期样本间差异表达基因,并对差异表达基因进行了GO功能和Pathway富集分析。GO功能分析结果显示,差异表达基因主要富集在跨膜转运、碳水化合物代谢途径和膜组分,它们协同调控为子实体生长发育提供稳定的内环境。KEGG富集分析结果表明,原基期上调的差异表达基因主要富集在核糖体蛋白和DNA复制,表明原基期细胞代谢旺盛,其中核糖体蛋白基因上调为后期蛋白质合成提供重要场所;采收期和开伞期子实体时期差异表达基因主要富集在碳水化合物代谢、脂肪酸降解和氨基酸代谢等途径,为巴氏蘑菇子实体的生长发育与成熟提供营养与能量。     

蝉棒束孢菌子实体对大鼠肾小管上皮细胞的影响

对蝉棒束孢菌子实体（0.75g/kg）重复灌胃SD雄性大鼠90d及恢复28d的早期肾损伤生物标记物肾损伤分子-1（KIM-1）和中性粒细胞明胶酶相关载脂蛋白（NGAL）进行测定,评估蝉棒束孢菌子实体对肾小管上皮细胞的影响;研究不同剂量蝉棒束孢菌子实体（0.25g/kg、0.5g/kg、1.0g/kg）对肾小管上皮细胞增殖和增生能力的影响。给药30、60、90d及恢复28d时,SD大鼠血清中KIM-1浓度与对照组相比均无显著差异（P>0.05）,给药30d、60d时,SD大鼠血清中NGAL浓度与对照组相比均无显著差异（P>0.05）,给药90d及恢复28d时,SD大鼠血清中NGAL浓度低于对照组（P<0.05）,且给药90d组与对照组相比有显著性差异（P<0.01）;免疫组化检测增殖细胞核抗原法（PCNA）及四甲基偶氮唑盐微量酶反应比色法（MTT）表明：与对照组相比,蝉棒束孢菌子实体能使肾小管上皮细胞增生能力增强,未导致肾小管上皮细胞凋亡。     

深挖垦复对锥栗重要农艺性状及土壤理化性质的影响

为探索锥栗林地高效的土壤管理方式,提升我国锥栗栽培管理技术水平,进而提高其产量、品质以及经济效益。该研究采用全垦和环垦两种方式对锥栗林地进行连续4年的深挖垦复,通过测定垦复前后土壤理化性质变化以及锥栗树体生长、叶片表型和生理特征、结果性状、产量及品质等重要农艺性状,统计数据并进行对比分析。结果表明:(1)深挖垦复对锥栗林地土壤理化性质改善效果显著,两种垦复方式土壤容重较垦复前降低31.21%及以上(0～30 cm处),土壤含水率、土壤孔隙度、有机质含量以及各种大量元素含量较垦复前和对照均有不同程度的增加,土壤肥力及其保水保肥能力显著增强。(2)环垦区土壤有机质含量、有效磷含量以及交换性镁含量高于全垦区,其土壤有机质含量较垦复前增加40.59%,远高于全垦增加幅度(17.76%),从土壤保肥能力的角度来看,环垦效果优于全垦。(3)土壤肥力的提升增强了其对锥栗叶片的供肥能力,使得叶片含水率、叶绿素含量以及各种矿质元素含量显著增加,从而提升其光合作用能力。(4)深挖垦复对锥栗树体生长、结实能力、产量及品质同样具有显著的提升效果,其中全垦和环垦区单位面积产量分别是对照的1.75倍和1.33倍,且栗苞总重、单果质量、出籽率、可溶性糖含量以及磷、钾元素含量显著高于对照,而空苞率显著低于对照。综上,深挖垦复是改良林地土壤和提高锥栗生产力的有效举措。     

Variation in Sexual Expression in Jacaratia mexicana (Caricaceae) in Southern Mexico: Frequency and Relative Seed Performance of Fruit-Producing Males

Dioecy, the segregation of male and female structures among individuals, is widespread in tropical plants, encompassing 10–30 percent of species in some sites. In many cases, interindividual sex separation is not complete, as individual plants, although nominally dioecious, may produce both types of reproductive structures. A common form of this sexual variation is the production of female structures in otherwise male individuals, commonly referred to as fruiting males. Here we report the existence of fruiting males in the dioecious tropical tree Jacaratia mexicana (Caricaceae). We show that fruiting males can constitute up to 45 percent of all males in some populations of a tropical forest in Southern Mexico. In order to determine the functional significance of fruiting males for the breeding system of J. mexicana , we compared the relative performance of male- and female-borne seeds. Our results show that seeds from fruiting males are three times less likely to germinate and survive than seeds from female trees. Based on relative seed fitness data, and sex ratios in natural populations, we estimate that 6–15 percent of the genes contributed by fruiting males to the next generation are transmitted via ovules, meaning that morphological variation in gender is at least partially accompanied by functional gender variation. Finally, our seed fitness estimates for fruiting males suggest that fruiting males will not replace female plants in natural populations.
Abstract in Spanish is available at http://www.blackwell-synergy.com/loi/btp .     

Expression and regulation of protein kinase CK2 during the cell cycle

There are indications from genetic, biochemical and cell biological studies that protein kinase CK2 (formerly casein kinase II) has a variety of functions at different stages in the cell cycle. To further characterize CK2 and its potential roles during cell cycle progression, one of the objectives of this study was to systematically examine the expression of all three subunits of CK2 at different stages in the cell cycle. To achieve this objective, we examined levels of CK2, CK2 and CK2 on immunoblots as well as CK2 activity in samples prepared from: (i) elutriated populations of MANCA (Burkitt lymphoma) cells, (ii) serum-stimulated GL30-92/R (primary human fibroblasts) cells and (iii) drug-arrested chicken bursal lymphoma BK3A cells. On immunoblots, we observed a significant and co-ordinate increase in the expression of CK2 and CK2 following serum stimulation of quiescent human fibroblasts. By comparison, no major fluctuations in CK2 activity were detected during any other stages during the cell cycle. Furthermore, we did not observe any dramatic differences between the relative levels of CK2 to CK2 during different stages in the cell cycle. However, we observed a significant increase in the amount of CK2 relative to CK2 in cells arrested with nocodazole. We also examined the activity of CK2 in extracts or in immunoprecipitates prepared from drug-arrested cells. Of particular interest is the observation that the activity of CK2 is not changed in nocodazole-arrested cells. Since CK2 is maximally phosphorylated in these cells, this result suggests that the phosphorylation of CK2 by p34cdc2 does not affect the catalytic activity of CK2. However, the activity of CK2 was increased by incubation with p34cdc2 in vitro. Since this activation was independent of ATP we speculate that p34cdc2 may have an associated factor that stimulates CK2 activity. Collectively, the observations that relative levels of CK2 increase in mitotic cells, that CK2 and CK2 are phosphorylated in mitotic cells and that p34cdc2 affects CK2 activity in vitro suggest that CK2 does have regulatory functions associated with cell division.