中国鞘寄蝇属的研究（双翅目：寄蝇科）

鞘寄蝇属Thecocarcelia全世界已记载7种,本文报道我国6种,其中2个新种。新种为:毛斑鞘寄蝇Thecocarcelia hirtmacula,多径鬃鞘寄蝇Th. setula。本文还编有种检索表。     

中国金绿寄蝇属记述：双翅目：寄蝇科

金绿寄蝇属Chrysocosmius在全世界已记载5种(古北界3种,东洋界2种),本文报道我国7种,其中包括4新种和2中国新纪录。新种为:巨眼鬃金绿寄蝇Chrysocosrmius ocellosetus,单鬃金绿寄蝇Chr.monostus,双齿金绿寄蝇Chr.bidentatus,亚合眼金绿寄蝇Chr.euholopticus。本文还编有种检索表。     

狭颊寄蝇属一新种记述（双翅目：寄蝇科）

本文中国发现的狭颊寄蝇属一新种宽属狭颊寄蝇。     

中国海南长足寄蝇属一新种(双翅目,寄蝇科)

长足寄蝇属幼虫主要寄生于土壤中生活的金龟总科昆虫,分布于东洋区、非洲热带区和古北区,其幼虫尾节背部均具2根特征性长鬃,区别于长足寄蝇族其它属而为一单系群.记述了采自我国海南省的长足寄蝇属1新种:海南长足寄蝇Dexia hainanensis sp.nov.,与分布东洋区的异长足寄蝇Dexia divergens Walker近似,但胸部背板黑色内侧纵条较窄,雌、雄腹部第3背板均具完整的1列后缘鬃,肛尾叶较窄.新种模式标本保存在沈阳师范大学昆虫研究所.     

中国俏饰寄蝇族的研究（双翅目：突颜寄蝇亚科）

本文记述中国寄蝇科、突颜寄蝇亚科、俏饰寄蝇族中的3属7种,其中包括1新属、2新纪录属和5新种,2新纪录种。     

中国蜉寄蝇属分类学研究(双翅目,寄蝇科)(英文)

蜉寄蝇属Phorocera隶属于双翅目Diptera寄蝇科Tachinidae追寄蝇业科Exoristinae追寄蝇族Exoristini,一般寄生于鳞翅口毒蛾科,夜蛾科和尺蛾科的幼虫;主要分布于古北区和新北区.该属区别于追寄蝇族Exoristini 其它属的特征为:眼后鬃列后方具黑毛,复眼具淡黄色长毛,单眼鬃位于前单眼后方,背中鬃3+3,翅内鬃0+3,腹部背板具心鬃.本文系统研究了中国蜉寄蝇属的4个已知种,勺肛蜉寄蝇P.assinilis,锥肛蜉寄蝇P.grandis,直条蜉寄蝇P.normalis和昏暗蜉寄蝇P.obscura;并首次描述了直条蜉寄蝇的雄性和采自我国辽宁本溪的1新种,辽宁蜉寄蝇Phorocera liaoningensis sp.nov.;编制了古北区本属6种雄性检索表.新种区别于近缘种勺肛蜉寄蝇的特征为:第4腹板后缘钝圆,中脉心角至中肘横脉的距离略长于心角至翅后缘的距离,雄性肛尾叶后面观端半部均匀变窄.     

中国寄蝇科一新纪录属及一新种(双翅目:寄蝇科)

本文记述在中国发现的寄蝇科一新纪录属,单寄蝇属Opsomeigemia和该属的一个新种,东方单寄蝇O.orientalis sp.nov.。     

中国丛毛寄蝇族一新属新种记述（双翅目：寄蝇科）

本文记述寄蝇科丛毛寄蝇族一新属,类梳寄蝇属Ｉｓｏｐｅｘｏｐｓｉｓ ｇｅｎ．ｎｏｖ．一新种,侧颜类梳寄蝇Ｉ．ｐａｒａｆａｃｉａｌｉｓ ｓｐ．ｎｏｖ．,并绘制了相应的特征图,模式标本保存于中国科学院动物研究所。     

中国贵州长腹寄蝇属三新种记述（双翅目：寄蝇科）

记述采自贵州地区的长腹寄蝇属Dolichocoxys Townsend 3个新种:黄基长腹寄蝇D. flavibasis sp. nov.、黑腹长腹寄蝇D. obscurus sp. nov.和短柄长腹寄蝇D. brevis sp. nov.。文中附所有新种的详细描述、鉴别特征图、近缘关系的讨论及中国长腹寄蝇属分种检索表。新种的模式标本保存于贵州省安顺市疾病预防控制中心医学昆虫研究室。     

中国菲寄蝇属分类研究(双翅目: 寄蝇科)

经研究发现中国菲寄蝇属现共有9种,其中包括4新种：金额菲寄蝇Phebellia aurifrons sp. nov.,褐粉菲寄蝇Ph. fulvipollinis sp. nov.,宽叶菲寄蝇Ph. latisurstyla sp. nov.和毛基节菲寄蝇Ph. setocoxa sp. nov.。我国新记录3种：叶蜂菲寄蝇Ph. clavellariae (Brauer & Bergenstamm),灰粉菲寄蝇Ph. glauca (Meigen)和拟灰粉菲寄蝇Ph. glaucoides Herting。本文除详细描述新种特征及绘制特征图外,还提供中国菲寄蝇属已知种类的分种检索表。     

Comprehensive separation and identification of chemical constituents from Apocynum venetum leaves by high-performance counter-current chromatography and high performance liquid chromatography coupled with mass spectrometry

High-performance counter-current chromatography (HPCCC) and high performance liquid chromatography coupled with mass spectrometry (HPLC-MS) was efficiently utilized for the separation and identification of the chemical components with a wide range of polarity from the mixed extract of Chinese medicinal herb Apocynum venetum. For HPCCC separation, four sets of solvent systems, n-hexane-ethyl acetate-acetonitrile-water (1.5:3.5:2:4.5, v:v:v:v), ethyl acetate-methanol-water (5:2:5, v:v:v) and n-butanol-methanol-water (5:1:5, v:v:v) were used for the one-step separation by four stages. The HPCCC separation was initiated by filling the column with the lower phase of n-hexane-ethyl acetate-acetonitrile-water (1.5:3.5:2:5, v:v:v:v) as a stationary phase followed by elution with the upper phase of n-hexane-ethyl acetate-acetonitrile-water (1.5:3.5:2:5, v:v:v:v) to separate the hydrophobic compounds (tail to head). Then the mobile phase was switched to the upper phase of ethyl acetate-acetonitrile-water (5:3:7, v:v:v) to eluted the moderate hydrophobic compounds, then the mobile phase was switched to the upper phase of ethyl acetate-methanol-water (5:2:5, v:v:v) to eluted the moderate hydrophilic compounds, and finally the hydrophilic compounds still retained in the column was eluted by the upper phase of n-butanol-methanol-water (5:1:5, v:v:v). A total of 16 named compounds including adhyperforin, hyperforin, amentoflavone, biapigenin, quercetin, avicularin, acetylated isoquercetin, acetylated hyperoside, astragalin, trifolin, isoquercetin, hyperoside, querciturone, rutin, chlorogenic acid and quercetin-3-O-β-D-glucosyl-β-D-glucopyranoside were successfully separated via the four sets of solvent systems in one step operation for 130 min. The compounds separated by HPCCC were identified by comparing with mixed standards data of HPLC-MS as well as NMR data.     

一种简便的肌醇磷脂微量分析方法

分析磷脂酰肌醇循环(PI cycle)的磷脂组分常采用双向薄层层析法．建立了一个简单快速的单向薄层层析分离肌醇磷脂方法．首先采用不同的有机溶剂体系分别提取非多磷酸肌醇磷脂和多磷酸肌醇磷脂,然后用不同的层析展开体系,对两部分磷脂进行单向薄层层析分离．采用无载体 ³²P标记实验对该方法分离效果进行了观察．此法适用于同位素标记和非标记样品中肌醇磷脂组分的比较分析及多磷酸肌醇磷脂的提取、纯化和定量．     

Sand dwelling Turbellaria from the Netherlands Delta area

Sand dwelling Turbellaria from the Delta of the Rivers Rhine, Meuse and Scheldt have been investigated. Thirty-eight samples taken from littoral and sublittoral stations in the Grevelingen, Eastern and Western Scheldt have been analysed.Thirty-three species were recorded (Acoela were not considered); twenty-four of them are new for the area and seven new species are described.Density and diversity of Turbellaria were higher in the Eastern Scheldt than in the Western Scheldt or in the Lake Grevelingen. A maximum density of 82 ind./100 cm³ was noted. A tentative calculation on relative abundance of the representatives of the different Turbellaria orders is established. Proseriata seem to be dominant in the localities studied.Abbreviations acg : accessory glands - aco : accessory organ - ad : atrial diverticle - b : bursa - br : brain - cil : cilia - cm : circular muscle - cn : cnidosac - co : copulatory organ - cs : cuticular spines - css : cuticular stylet sheat - de : ejaculatory duct - di : ductus intervesicularis - ds : seminal duct - dsp : spermatic duct - en : enteron - fd : female duct - fp : femal pore - ga : genital atrium - gf : glands in female duct - gg : glands - gp : genital pore - hp : adhesive papillae - ivs : intra capsular seminal vesicle - lm : longitudinal muscle - m : mouth - mp : male pore - ov : ovary - p : proboscis - pg : proboscisglands - ph : pharynx - phg : pharyngial glands - r : retractor muscle - rh : rhabdites - rhg : rhabdite glands - rs : seminal receptacle - s : stylet - sta : statocyst - ut : uterus - t : testis - v : vagina - vg : prostate vesicle - vi : vitellary - vs : seminal vesicle     

Double bond localization in minor homoallylic fatty acid methyl esters using acetonitrile chemical ionization tandem mass spectrometry

Double bond position in natural fatty acids is critical to biochemical properties, however, common instrument-based methods cannot locate double bonds in fatty acid methyl esters (FAME), the predominant analysis form of fatty acids. A recently described mass spectrometry (MS) method for locating double bonds in FAME is reported here for the analysis of minor (<1%) components of real FAME mixtures derived from three natural sources; golden algae (Schizochytrium sp.), primate brain white matter, and transgenic mouse liver. Acetonitrile chemical ionization tandem MS was used to determine double bond positions in 39 FAME, most at concentrations well below 1% of all fatty acid methyl esters. FAME identified in golden algae are 14:1n-6, 14:3n-3, 16:1n-7, 16:2n-6, 16:3n-6, 16:3n-3, 16:4n-3, 18:2n-7, 18:3n-7, 18:3n-8, 18:4n-3, 18:4n-5, 20:3n-7, 20:4n-3, 20:4n-5, 20:4n-7, 20:5n-3, and 22:4n-9. Additional FAME identified in primate brain white matter are 20:1n-7, 20:1n-9, 20:2n-7, 20:2n-9, 22:1n-7, 22:1n-9, 22:1n-13, 22:2n-6, 22:2n-7, 22:2n-9, 22:3n-6, 22:3n-7, 22:3n-9, 22:4n-6, 24:1n-7, 24:1n-9, and 24:4n-6. Additional FAME identified in mouse liver are 26:5n-6, 26:6n-3, 28:5n-6, and 28:6n-3. The primate brain 22:3n-7 and algae 18:4n-5 are novel fatty acids. These results demonstrate the usefulness of the technique for analysis of real samples. Tables are presented to aid in interpretation of acetonitrile CIMS/MS spectra.     

The influence of N-glycosylation and C-terminal sequence on secretion of HBV large surface antigen from S. cerevisiae

In Saccharomyces cerevisiae, we synthesized and secreted L-HBVsAg (named as pre-S(Met1 to Asn174)::S(Met175 to Ile400)) and three mutants, i.e., pre-S degree degree::S (Asn15Gln and Asn123Gln), pre-S degree degree::S degree (Asn15Gln, Asn123Gln, and Asn320Gln), and pre-S degree degree::S degree degree (Asn15Gln, Asn123Gln, Asn233Gln, and Asn320Gln). All of the secreted pre-S::S was N-glycosylated, i.e., hyper-mannosylated. In the secretion of pre-S degree degree::S and pre-S degree degree::S degree, besides the hyper-mannosylated form, another immunoreactive protein with much lower molecular mass was observed, which seems to be unglycosylated form of pre-S degree degree::S and pre-S degree degree::S degree. Only a part of the secreted pre-S degree degree::S or pre-S degree degree::S degree molecules was N-glycosylated, and the site for the partial N-glycosylation seems to be Asn233 in S-antigen region. Compared to the N-glycosylated pre-S degree degree::S and pre-S degree degree::S degree, pre-S degree degree::S degree degree (non-N-glycosylated mutant) was secreted with lower secretion efficiency but showed apparent immunoreactivity to anti-S antigen monoclonal Ab. Interestingly, unlike pre-S degree degree::S degree degree with authentic C-terminus, the recombinant pre-S degree degree::S degree degree with C-terminal myc or poly-histidine tag (pre-S degree degree::S degree degree::tag) was almost all aggregated into insoluble proteins in the intracellular region. Conclusively, the C-terminal sequence and glycosylation in S-antigen region seem to be of crucial importance in determining the secretion efficiency of L-HBVsAg in S. cerevisiae.     

Characteristics of Synthesis of Very-Long-Chain Saturated and Tetraenoic Fatty Acids in Swine Cerebral Microsomes

The elongation of arachidoyl-CoA (20:0-CoA) yielded 22:0 and 24:0 concomitantly, whereas the elongation of behenoyl-CoA (22:0-CoA) yielded only a negligible amount of 24:0 in adult swine cerebral microsomes. The dependence on time, pH, and the substrate concentrations were examined for the synthesis of 22:0 and 24:0 from 20:0-CoA. A microcomputer-aided simulation study suggested that there were two parallel pathways in the elongation of 20:0-CoA to 22:0 and 24:0. The elongation of 22:0-CoA could not be observed in adult swine cerebral microsomes; however, it was observed clearly in newborn swine and rat brain microsomes. A dilution experiment with the addition of cold 22:0-CoA in the reaction of elongation of 20:0-CoA confirmed the above suggestion that no intermediate 22:0 appeared during the synthesis of 24:0 from 20:0-CoA. The elongation of endogenous 20:4-CoA to 22:4 and 24:4 was examined in newborn swine cerebral microsomes, and the presence of two parallel pathways in the elongation of 20:4-CoA to 22:4 and 24:4 similar to those involved in the elongation of 20:0-CoA to 22:0 and 24:0 was suggested.     

栽培介质、营养液及化学药剂对红掌生长开花的影响

采用泥炭:珍珠岩:沙(1:1:1)、珍珠岩和水3种栽培介质及3个配方的营养液对红掌进行无土栽培,结果表明,以水作为介质,营养液配方为N:P₂O₅:K₂O=4:1:8的培养液对红掌株高、叶片数及植株净重的增加效果最好,但水培对红掌开花无促进作用。以水为介质的红掌经高温(32℃)胁迫后叶片黄化数为零,显著低于其它处理组;而在泥炭:珍珠岩:沙(1:1:1)介质中,则是6-BA处理的叶片黄化数明显低于其它处理组。     

三种控释肥在赤红壤中的氧化亚氮排放

采用静态箱收集和对比法,研究了无作物种植条件下包膜与否对高氮、均衡及高钾3种氮磷钾配比复合肥在华南赤红壤发育的菜园土中氧化亚氮(N2O)排放情况.结果表明:肥料氮磷钾配比不同,N2O排放量差异显著,3种类型复合肥N2O累积排放量表现为均衡型≥高氮型＞高钾型;同一类型复合肥,包膜控释能显著降低N2O排放量,包膜控释高氮、均衡及高钾型复合肥N2O排放总量分别为不包膜复合肥N2O排放量的34.4％、30.5％和89.3％;与不包膜相比,复合肥包膜能降低肥料在土壤中的N2O日排放通量,滞后和削减N2O排放高峰,减少土壤氮素损失以及由N2O排放造成的全球增温潜势.     

Bioactive compounds in plant materials for the prevention of diabetesand obesity

Plant materials have been widely studied for their preventive and therapeutic effects for type 2 diabetes mellitus (T2DM) and obesity. The effect of a plant material arises from its constituents, and the study of these bioactive compounds is important to achieve a deeper understanding of its effect at the molecular level. In particular, the study of the effects of such bioactive compounds on various biological processes, from digestion to cellular responses, is required to fully understand the overall effects of plant materials in these health contexts. In this review, I summarize the bioactive compounds we have recently studied in our research group that target digestive enzymes, dipeptidyl peptidase-4, myocyte glucose uptake, and lipid accumulation in adipocytes.

Abbreviations: AC: adenylyl cyclase; AMPK: AMP-activated protein kinase; βAR: β-adrenergic receptor; CA: catecholamine; cAMP: cyclic adenosine monophosphate; cGMP: cyclic guanosine monophosphate; DPP-4: dipeptidyl peptidase-4; ERK: extracellular signal-regulated kinase; GC: guanylyl cyclase; GH: growth hormone; GLP-1: glucagon-like peptide-1; GLUT: glucose transporter; HSL: hormone-sensitive lipase; IR: insulin receptor; IRS: insulin receptor substrate; MAPK: mitogen-activated protein kinase; MEK: MAPK/ERK kinase; MG: maltase-glucoamylase; NP: natriuretic peptide; NPR: natriuretic peptide receptor; mTORC2: mechanistic target of rapamycin complex-2; PC: proanthocyanidin; PI3K: phosphoinositide 3-kinase; PKA: cAMP-dependent protein kinase; PKB (AKT): protein kinase B; PKG: cGMP-dependent protein kinase; PPARγ: peroxisome proliferator-activated receptor-γ; SGLT1: sodium-dependent glucose transporter 1; SI: sucrase-isomaltase; T2DM: type 2 diabetes mellitus; TNFα: tumor necrosis factor-α.     

Xyloglucan structure and post-germinative metabolism in seeds of Copaifera langsdorfii from savanna and forest populations

The cotyledons of Copaifera langsdorfii Desf, have been shown to contain a water-soluble xyloglucan (amyloid), which represents about 40% of the seed's dry weight. On acid hydrolysis its composition (Glc:Xyl:Gal = 4.0:2.8–2.9:1.5–1.7) was similar to that of the well-characterized xyloglucan of Tamarindus indica L. (Glc:Xyl:Gal = 4.0:3.0–3.1:1.4). On hydrolysis with pure Trichoderma viride cellulase, both C. langsdorfii and T. indica xyloglucan gave the same xyloglucan oligosaccharides: but in significantly different proportions A:B₁:B₂:C = 1:0.4–0.5:2.1–2.2:3.1–3.4 in T. indica , and 1:1.1:1.8:7.4 and 1:1.3:2.6:12 for C. langsdorfii , savanna and forest populations respectively. This demonstrated a difference in fine molecular structure, notably in the distribution of the terminal non-reducing galactose substituents, between the xyloglucans of the two species and indicated differences in the specificities of their biosynthetic mechanisms. The xyloglucans obtained from C. langsdorfii seeds harvested from savanna and forest environments were slightly different, one from the other, in their sugar-residue composition (Glc:Xyl:Gal = 4.0:2.9:1.5 and 4.0:2.8:1.7, respectively), and were significantly different in the relative proportions of the xyloglucan oligosaccharides released on cellulase hydrolysis (above). Using light microscopy and biochemical methods, no difference in the pattern or rate of postgerminative xyloglucan metabolism was detected in seeds of savanna and forest origin. This is the first clear experimental evidence for differences in a storage xyloglucan structure between populations of the same species. It may indicate environmental influences on xyloglucan biosynthesis.