毛喉鞘蕊花的微量成分

从唇形科毛喉鞘蕊花全草的氯仿提取物分离到２个新的微量成分,鞘蕊花戊素和已素。基于光谱分析,鞘蕊花戊素和已 素的化学结构分别鉴定为１α,７β－二乙酰氧基－８,１３－环氧－６β羟基勒丹－１４烯－１１－酮（１）和７β－乙酰氧基－８,１３环氧－６β,α－二羟基勒丹－１４烯－１１－酮（２）。     

黄鞘蕊花的化学成分

从黄鞘蕊花(Coleus xanthanthus C. Y. Wuet Y. C. Huang)中分得8种成分。其中1个是新的醌式二萜,命名为黄鞘蕊花甲素,其结构为17-methyl(15→16)abieo-16-methoxy-2α-acetoxy-coleon U.7个已知化合物。coleon U(2),sugiol(3),β—谷甾醇,胡萝卜甙,三十三烷醇,三十三烷和二十八烷酸。     

毛喉鞘蕊花的化学成分

从毛喉鞘蕊花分离得到两个新二萜醌 :鞘蕊酮S(1) ,鞘蕊酮T(2 )和六个已知成分 :α 雪松醇 ,愈创木酚甘油醚 ,芫花素 ,鞘蕊醇B ,β 谷甾醇 ,豆甾醇。依据光谱和化学方法 ,它们的化学结构已被鉴定     

我国毛喉鞘蕊花的发掘与研究进展

本文介绍了哮喘病新药毛喉鞘蕊花的发掘过程,栽培条件下的形态特征和化学成分与印度毛喉鞘蕊花的区别,结果显示,二者并非同种植物,特将云南种定名为小江鞘蕊花。     

毛喉鞘蕊花化学及生理活性研究进展

本文简要综述了唇形科鞘蕊花属植物毛喉鞘蕊花(Coleus forskohlii(wild．)Briq．)化学及药理研究进展,尤其是二萜成分的研究状况。     

毛萼鞘蕊花甲素的结构

从毛萼鞘蕊花(Coleus esquirolii(L(?)vl. )Dunn.)的茎、叶中分离鉴定了一个新的二萜化合物,毛萼鞘蕊花甲素(对映-17-乙酰氧基-贝壳杉烷-16β-醇),和三个已知化合物,对映-贝壳杉烷-16p,17-二醇,齐墩果酸和β-谷甾醇。     

印产毛喉鞘蕊花的引种栽培研究

本文报道印产毛喉鞘蕊花肉质根稳定性状的分离及栽培技术路线．肉质根株提纯到９９．５％;求得了露地最佳效益种植法,最优水平搭配是：３０ｄ、１５株／ｍ２、高垄、覆膜、底肥、整枝、去花穗,产鲜根８７００ｋｇ／ｈｍ２．     

鞘蕊花的组织培养

植物名称鞘蕊花(Coleus forskohlii)。材料类别:顶芽、侧芽。培养条件:取鞘蕊花幼嫩的顶芽和侧芽,经自来水冲洗后去叶,用0.1％的升汞灭菌5min,再用无菌水冲洗数次后切成0.5～1.0cm长的带芽茎段,接入诱导培养基上。基本培养基为MS并附加不同浓度的BA,NAA和GA_3(单位mg/L);培养     

毛喉鞘蕊花愈伤组织的诱导及其活性成分的产生

本文简要报道了毛喉鞘蕊花(Coleus jorskohlii)无菌苗愈伤组织的诱导,初步培养及细胞悬浮培养,同时对培养细胞中的有效成分进行了初步分析。     

佛司可林类成分的光谱特征(一)

活性二萜佛司可林和异佛司可林已从毛喉鞘蕊花分离得到。本文详细描述了它们的光谱特征(包括一维和二维的核磁共振谱)。     

Mutation of invariant cysteines of mammalian metallothionein alters metal binding capacity, cadmium resistance, and 113Cd NMR spectrum.

Using a yeast expression vector system, we have expressed both wild type and six mutated Chinese hamster metallothionein coding sequences in a metal-sensitive yeast strain in which the endogenous metallothionein gene has been deleted. The mutant proteins have single or double cysteine to tyrosine replacements (C13Y, C50Y, and C13,50Y), single cysteine to serine replacements (C13S and C50S), or a single cysteine to alanine replacement (C50A). These proteins function in their yeast host in cadmium detoxification to differing extents. Metallothioneins which contain a cysteine mutation at position 50 (C50Y, C50S, C50A, and C13,50Y) conferred markedly less cadmium resistance than wild type metallothionein, or metallothionein with a single cysteine mutation at position 13 (C13Y and C13S). Wild type and three of the mutant Chinese hamster metallothioneins (C13Y, C50Y, and C13,50Y) were purified from yeast grown in subtoxic levels of either CdCl2 or 113CdCl2. All three of the mutant proteins bound less cadmium than the wild type protein when metal-binding stoichiometries were determined. The one-dimensional 113Cd NMR spectrum of the recombinant wild type Chinese hamster metallothionein was compared to the spectra of native rat and rabbit liver metallothioneins. The close correspondence between the 113Cd chemical shifts in these metallothioneins is consistent with the presence of two separate metal clusters, A and B, corresponding, respectively, to the alpha- and beta-domains, in the recombinant metallothionein. The one-dimensional 113Cd NMR spectra recorded on each of the three mutant metallothioneins, on the other hand, provide some indication as to the structural basis for the reduced, by one, metal stoichiometry of each of the mutant metallothioneins. For the C13Y mutant, it appears that the beta-domain now binds a total of two metal ions whereas with the C50Y mutant, the alpha-domain appears metal-deficient. For the double mutant, C13,50Y, the 113Cd resonances are indicative of major structural reorganizations in both domains.     

A Study on the Genus Gynostemma Bl. (Cucurbitaceae) from China

The genus Gynostemma B1. consists of 13 species and 2 varieties in the whole world, among which 11 species and 2 varieties occur in China. They are distributed in S. Shaanxi and the southern part of the Yangtze River (including Taiwan province) in China and also in Korea, Japan, Sri Lanka, India and Malesia. Based on the characters and dehiscence of fruit, the genus Gynostemma B1. may be divided into two subgenera, i.e. Subgen. I. Gynostemma and Subgen. II. Trirostllum (Z. P. Wang et Q. Z. Xie) C. Y. Wu ct S. K. Chen, comb. nov. 1. Subgenus Gynostemma. The fruits are baccate, globose, 3-umbonate and incorni culate on the apical side, indehiscent when mature. The style apex in female flower is bifid. Type of subgenus: Gynostemma pentaphyllum (Thunb.) Mak. This subgenus contains 8 species and 2 varieties in the world, among which 6 species and 2 varieties occur in China, i.e.1.G. simplicifolium B1. (Yunnan, Hainan of Guangdong); 2. G. laxum (Wall.) Cogn. (S. Yunnan, Hainan of Guangdong and Guangxi); 3. G. burmanicum King ex Chakr. (Yunnan), 3a. G. burmanicum var. molle C. Y. Wu (Yunnan); 4. G. pentaphyllum (Thunb.) Mak. (S. Shaanxi and the soutern area of the Yangtze River of China), 4a. G. pentaphyllum (Thunb.) Mak. var. dasycarpum C. V. Wu (Yunnan); 5. G. pubescens (Gagnep.) C. Y. Wu, st. nov. (Yunnan); 6. G. longipes C. Y. Wu, sp. nov. (endemic to China: Yunnan, Sichuan, Guizhou, Shaanxi and Guangxi). 2. Subgenus Trirostellum (Z. P. Wang et Q. Z. Xie) C. Y. Wu et S. K. Chen, comb. nov.——Trirostellum Z. P. Wang et Q. Z. Xie in Acta Phytotaxonomia Sinica 19 (4): 483. 1981, syn. nov. The fruit are capsules, subcampanulate, 3-corniculate on the apical side, dehiscent when mature. The style apex in female flower is luniform and irregularly denticulate at margin, rarely bifid. Type of subgenus: Gynostemma cardiospermum Cogn. ex Oliv. This subgenus comprises 5 species, which are all endemic to China. 1. G. yixingense (Z. P. Wang et Q. Z. Xie) C. Y. Wu et S. K. Chen (Jiangsu and Zhejiang); 2. G. cardio spermum Cogn. ex Oliv. (Hubei, Shaanxi and Sichuan); 3. G. microspermum C. Y. Wu et S. K. Chen (S. Yunnan); 4. G. aggregatum C. Y. Wu et S. K. Chen (NW. Yunnan); 5. G.laxiflorum C. Y. Wu et S. K. Chen (Anhui).     

Multinuclear magnetic resonance studies of the 2Fe.2S* ferredoxin from Anabaena species strain PCC 7120. 1. Sequence-specific hydrogen-1 resonance assignments and secondary structure in solution of the oxidized form

Complete sequence-specific assignments were determined for the diamagnetic 1H resonances from Anabaena 7120 ferredoxin (Mr = 11,000). A novel assignment procedure was followed whose first step was the identification of the 13C spin systems of the amino acids by a 13C(13C) double quantum correlation experiment [Oh, B.-H., Westler, M. W., Darba, P., & Markley, J. L. (1988) Science 240, 908-911]. Then, the 1H spin systems of the amino acids were identified from the 13C spin systems by means of direct and relayed 1H(13C) single-bond correlations [Oh, B.-H., Westler, W. M., & Markley, J. L. (1989) J. Am. Chem. Soc. 111, 3083-3085]. The sequential resonance assignments were based mainly on conventional interresidue 1H alpha i-1HNi + 1 NOE connectivities. Resonances from 18 residues were not resolved in two-dimensional 1H NMR spectra. When these residues were mapped onto the X-ray crystal structure of the homologous ferredoxin from Spirulina platensis [Fukuyama, K., Hase, T., Matsumoto, S., Tsukihara, T., Katsube, Y., Tanaka, N., Kakudo, M., Wada, K., & Matsubara, H. (1980) Nature 286, 522-524], it was found that they correspond to amino acids close to the paramagnetic 2Fe.2S* cluster. Cross peaks in two-dimensional homonuclear 1H NMR spectra were not observed for any protons closer than about 7.8 A to both iron atoms. Secondary structural features identified in solution include two antiparallel beta-sheets, one parallel beta-sheet, and one alpha-helix.     

Structure of the YSPTSPS repeat containing two SPXX motifs in the CTD of RNA polymerase II: NMR studies of cyclic model peptides reveal that the SPTS turn is more stable than SPSY in water.

The carboxyl-terminal domain of RNA polymerase II, which is rich in phosphorylation sites, contains 17--52 tandem repeats with the consensus sequence of the heptapeptide, YSPTSPS. The repeat unit of the heptapeptide has two SPXX motifs showing potential beta-turns, SPTS and SPSY. NMR studies were performed in water at pH 4.0 for two cyclic peptides containing one and two repeat units, cyclo-[C(1)R(2)D(3)Y(4)S(5)P(6)T(7)S(8)P(9)S(10)Y(11)S(12)R(13)D(14)C(15)] (peptide 1) and cyclo-[C(1)R(2)D(3)Y(4)S(5)P(6)T(7)S(8)P(9)S(10)Y(11)S(12)P(13)T(14)S(15)P(16)N(17)Y(18)S(19)R(20)D(21)C(22)] (peptide 2), which are cyclized with a disulfide bridge of two Cys residues at the N- and C-termini. SP in 1 and 2 are predominantly in trans form. The following NMR parameters were detected: (1) lower temperature coefficients of amide proton chemical shifts of T7 and S8 in 1, and Tx (T7 or T14), Sx (S8 or S15), Tz (T14 or T7) and Sz (S15 or S8) in 2, (2) significantly large deviation of H(alpha) chemical shifts from its random coil value (Delta H(alpha)) of Pro preceding the Thr (P6 in 1, and Px and Pz in 2), (3) relatively large (3)J(HNH alpha) coupling constants (>8.7 Hz) of T7 in 1 and Tx and Tz in 2, and (4) NOE (d(NN) (i, i+1)) connectivities between the amide protons of T7-S8 and S10-Y11 in 1, and Tx-Sx, S10-Y11, Tz-Sz, and N17-Y18 in 2, although two Pro-Thr-Ser segments in 2 (each of these are annotated by 'x' and 'z') in the first and second repeat units were not distinguishable. Comparison of the NMR parameters between the cyclic peptides and the corresponding linear peptides indicates that cyclization promotes structural stabilization in water. The present NMR data were consistent with the presence of a beta-turn at both SPTS and SPSY: S(5)P(6)T(7)S(8) and S(8)P(9)S(10)Y(11) in 1, and SPxTxSx, SPzTzSz, SP(9)S(10)Y(11), SP(16)N(17)Y(18) in 2. However, the structure of the SPTS segment is more stable than that of the SPSY segment. Conformations consistent with NMR parameters including NOE distances were obtained through molecular dynamics and energy minimization methods. These calculations yielded two stable conformers for the SPTS segment. One of the two corresponds to a type I beta-turn.     

Structural analysis of a new glycosphingolipid from the lipopolysaccharide-lacking bacterium Sphingomonas adhaesiva.

A new glycosphingolipid, GSL-4B, was isolated from Sphingomonas adhaesiva and found to share the ceramide moiety with GSL-1 and GSL-3 from Sphingomonas capsulata studied earlier [Kawahara, K.; Moll, H.; Knirel, Y. A.; Seydel, U.; Z?hringer, U. Eur. J. Biochem. 2000, 267, 1837-1846]. It is heterogeneous with respect to the long-chain bases erythro-2-amino-1,3-octadecanediol (sphinganine), (13Z)-erythro-2-amino-13-eicosene-1,3-diol, and (13Z)-erythro-2-amino-13,14-methylene-1,3-eicosanediol which in GSL-4B are present in the ratios of 1.1:1.0:1.1, and all bearing amide-linked (S)-2-hydroxymyristic acid. Methylation analysis and MALDI-TOF-MS along with 1H and 13C NMR spectroscopy showed that the carbohydrate part of GSL-4B has the structure of alpha-D-Glcp-(1-->4)-alpha-D-Galp-(1-->6)-alpha-D-Glcp-(1-->4)-alpha-D-GlcpA-(1-->1)-Cer     

Immunochemical characterization of Neisseria meningitidis serotype antigens by immunodiffusion and SDS-polyacrylamide gel electrophoresis immunoperoxidase techniques and the distribution of serotypes among cases and carriers

The chemical nature of the antigens of the meningococcal serotypes described by Frasch and colleagues was determined by a combination of immunodiffusion and the SDS-polyacrylamide gel electrophoresis immunoperoxidase technique (SGIP). It was confirmed that the serotype antigens of the outer membrane of serotypes 1, 2, 6, 9, 11 and 12 were proteins, whilst those of serotypes 4,5 and 8 were lipopolysaccharides. Serotype 2 can now be divided into three related types, provisionally called 2a (originally serotype 2), 2b and 2c with the specific antigens being proteins having molecular weights of 41,000, 41,500 and 41,500, respectively. A total of 195 strains of meningococci isolated from patients and carriers in the Netherlands and 20 serogroup Y strains from patients in the U.S.A. were serotyped by means of immunodiffusion. Serotype 2a could be demonstrated in some strains belonging to the serogroups B (only those from carriers), C, W-135 and Y (only those from the U.S.A.). The W-135 strains isolated from patients in this series more often belonged to serotype 2a than did the W-135 strains from carriers. Serotype 2b was present in about half of the serogroup B and a few serogroup C strains isolated from patients with meningitis, but absent in serogroup B and C strains from carriers. Serotype 2c could only be demonstrated in serogroup Y strains, both from the Netherlands and the U.S.A. The other serotypes were found only sporadically.     

五福花科的初步研究

本文对五福花科的分类进行了初步研究,提出了新的分类系统,并对其系统演化规律、地理分布等进行了讨论。     

Biochar-Induced Priming Effects in Young and Old Poplar Plantation Soils

The priming effect (PE) induced by biochar provides a basis for evaluating its carbon (C) sequestration potential in soils. A 60 days’ laboratory incubation was conducted, which involved the amendment of biochar (1% of soil mass) produced from rice straw at 300ºC (B300) and 500ºC (B500) to young (Y) and old (O) poplar plantation soils, with the aim of studying the responses of biochar-induced PEs to poplar plantation ages. This incubation included six treatments: Y + CK (control), Y + B300, Y + B500, O + CK, O + B300, and O + B500. Carbon dioxide (CO₂) emissions were significantly increased (p < 0.05) in the B300 amended soils, while it was decreased in the B500 amended soils compared to the CK. The primed CO₂ emissions were 2.35 times higher in the Y + B300 than the O + B300 treatments, which was measured to be 18.6 and 5.56 mg C·kg^-1 with relative PEs of 12.4% and 3.35%, respectively. However, there was little difference between the primed CO2 emissions in Y + B500 and O + B500 treatments, which were measured to be -24.9 and -29.6 mg·C·kg^-1 with relative PEs of -16.6% and -17.8%, respectively. Dissolved organic carbon (DOC) was significantly lower in the young poplar plantation soil than that in the old poplar plantation soil regardless of biochar amendment throughout the incubation, indicating greater C-limit of soil microorganisms in the young poplar plantation soil. Using ¹³C isotope tracing, neither B300 nor B500 decreased native soil-derived DOC, which indicated that the negative B500-induced PEs were not due to a reduction in the availability of native soil-derived C. In conclusion, the response of biochar-induced PEs to poplar plantation age depends on biochar types while soil available C indirectly affects biocharinduced PEs. Further studies should focus on how the interactive effects between soil C availability and microbial community impacts biochar-induced PEs.     

Role of the P2Y12 receptor in the modulation of murine dendritic cell function by ADP

The effects of ADP on the biology of dendritic cells have been studied much less than those of ATP or adenosine. In this study, we showed that adenosine-5'-O-(2-thiodiphosphate) (ADPβS) induced intracellular Ca(2+) transients in murine dendritic cells (DCs). This effect was abolished by AR-C69931MX, a dual P2Y(12) and P2Y(13) receptor antagonist. RT-PCR experiments revealed the expression of both P2Y(12) and P2Y(13) mRNA in DCs. The Ca(2+) response to ADPβS was maintained in P2Y(13)-deficient DCs, whereas it was abolished completely in P2Y(12)(-/-) DCs. ADPβS stimulated FITC-dextran and OVA capture in murine DCs through macropinocytosis, and this effect was abolished in P2Y(12)(-/-) DCs. ADPβS had a similar effect on FITC-dextran uptake by human monocyte-derived DCs. OVA loading in the presence of ADPβS increased the capacity of DCs to stimulate OVA-specific T cells, whereas ADPβS had no effect on the ability of DCs to stimulate allogeneic T cells. Moreover, after immunization against OVA, the serum level of anti-OVA IgG1 was significantly lower in P2Y(12)(-/-) mice than that in wild-type controls. In conclusion, we have shown that the P2Y(12) receptor is expressed in murine DCs and that its activation increased Ag endocytosis by DCs with subsequent enhancement of specific T cell activation.     

Transmembrane domains 4, 5, 7, 8, and 10 of the human reduced folate carrier are important structural or functional components of the transmembrane channel for folate substrates

The human reduced folate carrier (hRFC) facilitates membrane transport of folates and antifolates. hRFC is characterized by 12 transmembrane domains (TMDs). To identify residues or domains involved in folate binding, we used substituted cysteine (Cys) accessibility methods (SCAM) with sodium (2-sulfonatoethyl)methanethiosulfonate (MTSES). We previously showed that residues in TMD11 of hRFC were involved in substrate binding, whereas those in TMD12 were not (Hou, Z., Stapels, S. E., Haska, C. L., and Matherly, L. H. (2005) J. Biol. Chem. 280, 36206-36213). In this study, 232 Cys-substituted mutants spanning TMDs 1-10 and conserved stretches within the TMD6-7 (residues 204-217) and TMD10-11 connecting loop domains were transiently expressed in hRFC-null HeLa cells. All Cys-substituted mutants showed moderate to high levels of expression on Western blots, and only nine mutants including R133C, I134C, A135C, Y136C, S138C, G163C, Y281C, R373C, and S313C were inactive for methotrexate transport. MTSES did not inhibit transport by any of the mutants in TMDs 1, 3, 6, and 9 or for positions 204-217. Whereas most of the mutants in TMDs 2, 4, 5, 7, 8, and 10, and in the TMD10-11 connecting loop were insensitive to MTSES, this reagent inhibited methotrexate transport (25-75%) by 26 mutants in these TMDs. For 13 of these (Y126C, S137C, V160C, S168C, W274C, S278C, V284C, V288C, A311C, T314C, Y376C, Q377C, and V380C), inhibition was prevented by leucovorin, another hRFC substrate. Combined with our previous findings, these results implicate amino acids in TMDs 4, 5, 7, 8, 10, and 11, but not in TMDs 1, 2, 3, 6, 9, or 12, as important structural or functional components of the putative hydrophilic cavity for binding of anionic folate substrates.