Inhibitor and substrate activities of sesquiterpene olefins toward (+)-δ-cadinene-8-hydroxylase, a cytochrome P450 monooxygenase (CYP706B1)

Several lines of evidence indicate that (+)-δ-cadinene-8-hydroxylase (CYP706B1) plays an important role in biosynthesis of gossypol in Gossypium arboreum L. ( [Luo et al., 2001] and [Wang et al., 2003]). The catalytically active enzyme has been expressed in yeast microsomes. Some microsomal preparations conjugated the hydroxylated (+)-δ-cadinene to a moiety that has not yet been identified. However, when microsomes were treated with n-octyl-β-d-glucoside (OG), a non-ionic detergent, (+)-δ-cadinene was reproducibly converted to the free alcohol, 8-hydroxy-(+)-δ-cadinene. OG had little effect on K_m and slightly stimulated apparent V_max. Enzymic activity was more than 10-fold more sensitive to inhibition by the N-substituted imidazole clotrimazole than to miconazole. Sesquiterpene olefins (−)-δ-cadinene, (−)-α-cubebene, (−)-α-muurolene, α-humulene, and a mixture of (−)- and (+)-α-copaene were inhibitory to hydroxylation of (+)-δ-cadinene. In addition, (−)-α-cubebene, (−)-α-muurolene, α-humulene, and, to a smaller extent, (−)-δ-cadinene served as alternative substrates for (+)-δ-cadinene-8-hydroxylase and were converted to mono-hydroxylated products. Of the five olefins tested, α-humulene and α-copaene are found in lysigenous glands of cotton (Elzen et al., 1985), which are also the site of gossypol accumulation ( [Bell et al., 1978] and [Mace et al., 1976]) and the probable site of its biosynthesis.     

阳际峰自然保护区地面生苔藓植物分布与环境因子关系研究

在江西阳际峰自然保护区调查的25个样地中,共采集到地面生苔藓植物34科56属106种（包括1变种）。应用CCA排序法,首次定量分析了该区38种主要地面生苔藓植物与环境因子的关系。结果表明,苔藓植物的分布和生物多样性受环境因子的影响较大,湿度、基质是影响地面生苔藓植物分布的主要环境因子,其他影响因子依次为乔木郁闭度、灌木盖度、海拔高度、人为干扰和坡度。     

不同种源厚朴苗期性状变异及主成分分析

基于厚朴（Magnolia officinalis）作为一种传统中药植物及分布区域广、环境异质化程度明显的现象,采用田间种源实验,对分布在中国7个省的14个种源厚朴苗期的生长性状进行了观测分析。结果表明,不同种源厚朴的苗期生长性状差异显著。种源遗传力分析表明,苗高和单株叶面积两个性状的遗传力较高,分别为0.93、0.79,可认为以苗高和单株叶面积为主的种源多性状综合选择改良潜力巨大。相关性分析表明各性状间遗传相关、表型相关、环境相关均存在一定的相关关系,单株叶面积和地上部生长性状的遗传相关程度高于地下部生长性状,表型显著相关的性状组合数量和程度低于遗传相关。厚朴苗期种源选择的首选因子为各生物量及单数叶面积性状,辅助因子为苗高和地径。通过系统聚类分析,初步选定景宁、武夷山、龙胜、开县、城固、宁强及洋县的种源为优良厚朴种源。     

电刺激迷走神经对蟾蜍心率和心率变异的影响

目的:观察不同频率迷走神经刺激对蟾蜍离体心脏的心率及心率变异的影响。方法:将蟾蜍心脏和右侧迷走交感干离体后,以不同频率电刺激神经,记录心电图曲线并作心率变异性(HRV)分析。结果:交感神经阻断后,电刺激迷走交感干,心率(HR)显著下降(P0.01),全部正常心动周期的标准差(SDNN)和相邻正常心动周期差值的均方根(RMSSD)显著升高(P0.01),不同频率刺激组之间没有明显差异;与对照组相比,各指标变化较大;给药组0.2Hz时高频(HF)显著升高(P0.01),低频/高频比值(LF/HF)明显降低(P0.05),0.8Hz时HF和LF/HF接近刺激前水平。结论:一定范围内增加刺激频率,迷走神经降低心率的作用增强;没有交感神经调节条件下的迷走神经对心率和心率变异的调节可能存在不同的机制。     

下坡跑后大鼠腓肠肌成肌调节因子的变化

目的:探讨成肌调节因子(MyoD)在肌肉损伤修复过程中的动态表达,为促进运动肌肉损伤的再生修复提供实验依据。方法:将健康雄性2月龄SD大鼠80只,随机分为对照组(n=10)和下坡运动组(n=70),下坡运动组再分为运动后即刻组、12h、24h、48h、72h、7d和14d组,各运动组动物均进行持续性下坡跑,分别在运动结束后8个时间点麻醉,下腔静脉取血,分离血清,取双侧腓肠肌。常规检测CK、LDH的活性。采用免疫组织化学染色法以及计算机图像分析技术定量统计MyoD因子表达情况。结果:血清CK、LDH在运动后即刻显著上升,后逐渐下降至正常水平。成肌调节因子MyoD在正常骨骼肌中即有表达,各运动组大鼠腓肠肌MyoD因子表达较对照组均有增加,48h组大鼠腓肠肌MyoD免疫阳性细胞核数明显多于对照组(P0.05),后随时间逐渐下降。结论:离心运动后即刻MyoD的表达水平开始上升,48h达到峰值,随后逐渐下降至正常水平。提示成年早期大鼠(2月龄)已具备较成熟的肌肉再生修复能力。     

选择性雌激素受体调节剂

雌激素替代疗法（estrogen replacement therapy,ERT）是治疗绝经后综合征的首选治疗方案,但是长期应用导致子宫内膜增生、乳腺癌等。选择性雌激素受体调节剂主要通过ER亚型、共调节子、靶启动子、雌激素受体相关受体等机制实现其组织选择性,在发挥骨骼、心血管保护作用的同时,减少了对乳腺及生殖系统的副作用。目前,选择性雌激素受体调节剂的种类、作用的组织特异性及其临床应用在医学界引起广泛关注,具有广阔的发展前景。     

10-Phenyl-[11]-cytochalasans from Indonesian mushroom Microporellus subsessilis

10-Phenyl-[11]-cytochalasans (4-6), together with three known derivatives (1-3), were isolated from the MeOH extract of the Indonesian mushroom Microporellus subsessilis by a bioassay-guided fractionation. The compounds 6 and 1-3 induced immotility in Artemia salina.     

实验性急性肝衰竭大鼠血清中TNF-α的来源及水平变化

目的研究D-氨基半乳糖／内毒素所致大鼠急性肝衰竭模型中血清内TNF-α的来源及不同时间点的水平变化。方法取30只Wistar大鼠腹腔内注射D-氨基半乳糖／内毒素诱导大鼠急性肝衰竭模型（AHF组,n=30）,于建模3h、6h、12h、24h、48h、72h各取5只动物检测其血清丙氨酸转氨酶（ALT）与肝组织的病理形态学变化;采用ELISA检测不同时间点动物血清中TNF-α水平的变化;通过免疫组化法检测不同时间点动物肝、肺组织内TNF-α的表达。另取30只Wistar大鼠腹腔内注射等量生理盐水为正常对照（N组,n=30）。结果AHF组各时间点血清ALT的增高与N组相比有统计学差异（P〈0．05）,肝脏内炎细胞浸润、坏死明显;AHF组与N组相比血清内TNF-α的增高在3h（P〈0．01）、6h（P〈0．05）有统计学差异;AHF组肺组织与N组相比TNF-α的表达在3h、6h、12h（均为P〈0．01）有统计学差异。结论本实验成功建立了大鼠AHF模型;TNF-α在此模型的早期阶段起重要作用;肺脏可能是血清内TNF-α的主要来源之一。     

Exchange of active site residues alters substrate specificity in extremely thermostable β-glycosidase from Thermococcus kodakarensis KOD1

β-Glycosidase from Thermococcus kodakarensis KOD1 is a hyperthermophilic enzyme with β-glucosidase, β-mannosidase, β-fucosidase and β-galactosidase activities. Sequence alignment with other β-glycosidases from hyperthermophilic archaea showed two unique active site residues, Gln77 and Asp206. These residues were represented by Arg and Asp in all other hyperthermophilic β-glycosidases. The two active site residues were mutated to Q77R, D206N and D206Q, to study the role of these unique active site residues in catalytic activity and to alter the substrate specificity to enhance its β-glucosidase activity. The secondary structure analysis of all the mutants showed no change in their structure and exhibited in similar conformation like wild-type as they all existed in dimer form in an SDS-PAGE under non-reducing conditions. Q77R and D206Q affected the catalytic activity of the enzyme whereas the D206N altered the catalytic turn-over rate for glucosidase and mannosidase activities with fucosidase activity remain unchanged. Gln77 is reported to interact with catalytic nucleophile and Asp206 with axial C2-hydroxyl group of substrates. Q77R might have made some changes in three dimensional structure due to its electrostatic effect and lost its catalytic activity. The extended side chains of D206Q is predicted to affect the substrate binding during catalysis. The high-catalytic turn-over rate by D206N for β-glucosidase activity makes it a useful enzyme in cellulose degradation at high temperatures.     

Guanine Nucleotide Exchange Factor αPIX Leads to Activation of the Rac 1 GTPase/Glycogen Phosphorylase Pathway in Interleukin (IL)-2-stimulated T Cells

Recently, we have reported that the active form of Rac 1 GTPase binds to the glycogen phosphorylase muscle isoform (PYGM) and modulates its enzymatic activity leading to T cell proliferation. In the lymphoid system, Rac 1 and in general other small GTPases of the Rho family participate in the signaling cascades that are activated after engagement of the T cell antigen receptor. However, little is known about the IL-2-dependent Rac 1 activator molecules. For the first time, a signaling pathway leading to the activation of Rac 1/PYGM in response to IL-2-stimulated T cell proliferation is described. More specifically, αPIX, a known guanine nucleotide exchange factor for the small GTPases of the Rho family, preferentially Rac 1, mediates PYGM activation in Kit 225 T cells stimulated with IL-2. Using directed mutagenesis, phosphorylation of αPIX Rho-GEF serines 225 and 488 is required for activation of the Rac 1/PYGM pathway. IL-2-stimulated serine phosphorylation was corroborated in Kit 225 T cells cultures. A parallel pharmacological and genetic approach identified PKCθ as the serine/threonine kinase responsible for αPIX serine phosphorylation. The phosphorylated state of αPIX was required to activate first Rac 1 and subsequently PYGM. These results demonstrate that the IL-2 receptor activation, among other early events, leads to activation of PKCθ. To activate Rac 1 and consequently PYGM, PKCθ phosphorylates αPIX in T cells. The biological significance of this PKCθ/αPIX/Rac 1 GTPase/PYGM signaling pathway seems to be the control of different cellular responses such as migration and proliferation.