植物乙酰辅酶A羧化酶β亚基acc D在因研究进展

综述了乙酰辅酶A羧化酶及其催化域羧基转移酶(Carboxyltransferase,CT)的β亚基(β-CT)的分布和生理功能、β-CT编码基因accD的分子生物学特征及乙酰辅酶A羧化酶在脂肪酸代谢工程中的应用研究进展。     

17β-雌二醇对AC细胞活性、细胞周期和超微结构的影响

通过免疫荧光获得雌激素α、β受体在体外星形胶质细胞（Acrocyte,AC）中表达的形态学证据;CCK-8法获得脂多糖（Lipopolysaccharide,LPS）激发AC的适宜浓度。在此基础上,研究了17β-雌二醇（17β-estradiol,E2）对AC的细胞活性、细胞周期和超微结构的影响。结果显示：E2作用AC 48h,10nmol/L E2可提高AC细胞活性和G2＋S%（P〈0.05）,而100,1 000nmol/L E2可降低AC细胞活性（P〈0.05）,100nmol/L E2还可降低G2＋S%（P〈0.05）;100nmol/L E2作用AC 24,48,72h,均可降低AC细胞活性和G2＋S%,以作用48h时抑制作用最强（P〈0.05）;10nmol/L E2可引起AC线粒体数量增加,细胞核分裂增多,但线粒体、粗面内质网结构正常,而100nmol/L E2可导致AC线粒体肿胀或空泡化,粗面内质网扩张或断裂。结果表明,低浓度（10nmol/L）E2促进AC增殖;高浓度（100,1 000nmol/L）E2抑制AC增殖。     

Modelling the β-amylase activity during red sorghum malting when Bacillus subtilis is used to control mould growth

Steeping in dilute alkaline (0.2% NaOH) followed by resteeping in biocontrol (starters of Bacillus subtilis S499) has been used during red sorghum malting. The effect of steeping and germination conditions has been described using 2 functions: a Weibull 4-parameter model combined with a General Linear Model with Logarithm Link with significant goodness. Steeping conditions (combined use of NaOH and B. subtilis S499) affects the synthesis capacity of grain: when B. subtilis culture used in the steeping step is diluted, ln α increases, suggesting a loss of treatment efficacy. The germination temperature affects the β-amylase synthesis rate during the induction phase: the germination temperature increase is accompanied by a decrease of the β-amylase synthesis rate. During the repression phase of β-amylase synthesis, the effect of malting conditions was found to taper.     

水溶性烯丙孕素-磺丁基-β-环糊精包合物的制备及表征

旨在提高烯丙孕素原药在水中的溶解度,提高烯丙孕素原药的生物利用度,使用磺丁基-β-环糊精对烯丙孕素原药进行包合。本试验使用冷冻干燥法来制备烯丙孕素-磺丁基-β-环糊精包合物,以此来解决烯丙孕素在临床使用中因其水不溶性而受到限制及其使用后生物利用度低的问题,进而拓宽烯丙孕素的药用途径。通过傅里叶变换红外光谱法、热重分析法和显微镜成像法对所制得的烯丙孕素包合物进行表征,并用溶解度法对包合物进行溶解度测定。以包合物的收率和包合率为评价指标,筛选最优的包合物制备条件。结果显示：经筛选,包合物的最佳制备条件：在55℃,ALT与SBE-β-CD的投料摩尔比为1：6,包合时间为5 h,溶液pH为8,溶剂量为15 mL（当以ALT投药量为0.1 g时计）;以最优制备条件制备所得的包合物中ALT的平均包合率为（90.90±1.80）%（n=3）,平均载药量为（4.30±2.30）%（n=3）,包合物的收率为（93.19±1.67）%。经傅里叶变换红外光谱法、热重分析法和显微镜成像法对所制得的包合物进行表征,可证实成功制得包合物。溶解度法试验结果表明,形成包合物后,其溶解度较烯丙孕素原药提高了988.86倍,且该包合物稳定性好,可满足不同剂型的要求。磺丁基-β-环糊精对烯丙孕素原药具有较好的增溶作用,达到了增加药物溶解度的目的,且该制备方法简单,条件温和,易于产业化生产,有利于烯丙孕素的进一步开发利用。     

Effect of Estradiol-17β on protein synthesis and degradation rates in fused bovine satellite cell cultures

Although androgenic and estrogenic steroids are widely used to enhance muscle growth and increase feed efficiency in feedlot cattle, their mechanism of action is not well understood. Further, in vivo studies indicate that estradiol (E2) affects muscle protein synthesis and/or degradation, but in vitro results are inconsistent. We have examined the effects of E2 treatment on protein synthesis and degradation rates in fused bovine satellite cell (BSC) cultures. Additionally, to learn more about the mechanisms involved in E2-enhanced muscle growth, we have examined the effects of compounds that interfere with binding of E2 or insulin-like growth factor (IGF)-1 to their respective receptors on E2-induced alterations in protein synthesis and degradation rates in BSC cultures. Treatment of fused BSC cultures with E2 results in a concentration-dependent increase (P < 0.05) in protein synthesis rate and a decrease (P < 0.05) in protein degradation rate. The pure estrogen antagonist ICI 182 780 suppresses (P < 0.05) E2-induced alterations in protein synthesis and degradation in fused BSC cultures. The G-protein coupled receptor (GPR)-30 agonist G1 does not affect either synthesis or degradation rate, which establishes that GPR30 does not play a role in E2-induced alterations in protein synthesis or degradation. JB1, a competitive inhibitor of IGF-1 binding to the Type 1 insulin-like growth factor receptor (IGFR-1), suppresses (P < 0.05) E2-induced alterations in protein synthesis and degradation. In summary, our data show that E2 treatment directly alters both protein synthesis and degradation rates in fused BSC cultures via mechanisms involving both the classical estrogen receptor (ER) and IGFR-1.     

Wnt/β-catenin信号通路上游基因在山羊绒周期性再生及着色过程中的表达分析

为初步探究Wnt/β-catenin信号通路是否参与山羊绒周期性再生及着色过程,本试验采用实时荧光定量技术对Wnt/β-catenin信号通路上游基因β-catenin、Lef1/Tcf3及该通路拮抗基因Dkk1mRNA在白色绒山羊绒毛生长不同时期及黑、白色绒山羊绒毛生长旺盛期时体侧部皮肤组织中的相对表达量进行研究。结果显示,上述通路中β-catenin、Lef1/Tcf3基因mRNA在白色绒山羊不同时期体侧部皮肤组织中的相对表达量具有明显变化规律即生长前期缓慢上调,旺盛期时表达量最高,生长后期及退行期逐渐下调,休止期表达量最低;Dkk1基因mRNA在白色绒山羊不同时期体侧部皮肤组织中的相对表达量则无明显规律性。上述各基因mRNA在黑、白色绒山羊生长旺盛期时体侧部皮肤组织中的相对表达量并无显著差异(P0.05)。结果提示,Wnt/β-catenin信号通路参与山羊绒周期性再生过程,但该通路并不涉及生长旺盛期时绒毛的着色过程。     

超高效液相色谱法测定饲料中斑蝥黄和β-阿朴-8’-胡萝卜素酸乙酯含量方法的研究

为有效快速测定饲料中斑蝥黄和β-阿朴-8’-胡萝卜素酸乙酯含量,饲料经甲醇、正己烷和乙酸乙酯混合液萃取后,在氮气保护下浓缩,用甲基叔丁基醚-乙腈溶液复溶,注入超高效液相色谱仪中进行测定。结果表明:斑蝥黄浓度为1.25~10.0μg/mL,β-阿朴-8’-胡萝卜素酸乙酯为2.50~20.0μg/mL线性关系良好;斑蝥黄和β-阿朴-8’-胡萝卜素酸乙酯的检测限为0.06 mg/kg,定量限为0.20 mg/kg。斑蝥黄5个添加水平的平均回收率为72.8%~82.8%,相对标准偏差(RSD)为0.41%~1.06%;β-阿朴-8’-胡萝卜素酸乙酯5个添加水平的平均回收率为72.0%~82.8%,RSD为0.46%~1.41%。说明该方法简便、快速、灵敏度高、准确度好,适用于测定饲料中斑蝥黄和β-阿朴-8’-胡萝卜素酸乙酯含量。     

利用凝胶扩散法测定刺萼龙葵种子中β-甘露聚糖酶的活性

β-甘露聚糖酶是种子萌发过程中降解胚乳细胞壁的关键酶,明确其活性的动态变化可为揭示杂草种子的休眠萌发机制提供重要依据。以外来杂草刺萼龙葵Solanum rostratum Dunal种子为材料,建立了种子中β-甘露聚糖酶活性的检测方法—凝胶扩散法。利用凝胶扩散法对不同贮存时间及贮存条件下刺萼龙葵种子中β-甘露聚糖酶的活性进行了检测,发现贮存3年以上的种子中该酶的活性为0.03 nmol/(min·mg),显著低于贮存3年以下的种子中的酶活性0.15 nmol/(min·mg),而湿润冷藏的种子中β-甘露聚糖酶的活性为0.12 nmol/(min·mg),显著高于干燥冷藏的种子的酶活性0.02 nmol/(min·mg)。实际应用结果表明,凝胶扩散法综合了传统方法的优势,检测特异性强、灵敏度高、重复性好,可同时检测大量种子样品,具有良好的实用性。     

Uterine Expression of WNT7A and β-catenin After Induction of Oestrus in Sheep

WNT7A and β-catenin localisations and roles in regulating periimplantation ovine conceptus development under natural estrous conditions have been elaborated.However,their locations and expression patterns have not been reported under induction of oestrus.The localisation,expression and function of WNT7A and β-catenin in the uterine tissues of the early pregnant and non-pregnant sheep on days 10,12,14,16 and 18 following artificial induction of oestrus were investigated by means of in situ hybridisation,real-time RT-PCR,immuno-histochemistry and western blotting methods.WNT7A and β-catenin mRNA and protein were both restricted to the apical surfaces of the uterine luminal epithelium (LE) and glandular epithelium (GE).In pregnant sheep,protein localisation of WNT7A and β-catenin was observed both in the endometrial LE and GE.Their staining presented on day 10,increased between day 12 and day 16,and decreased on day 18.WNT7A and β-catenin mRNA and protein expression increased initially and then decreased from day 10 to day 18,peaking on day 16,and β-catenin reaching a peak on day 18 in the uterine tissues of pregnant sheep (p0.05).By contrast,no significant changes in WNT7A and β-catenin mRNA and protein expression levels were observed from day 10 to day 18 of the oestrus cycle in the uterine tissues of non-pregnant sheep (p0.05).Additionally,WNT7A and β-catenin mRNA and protein expression levels in the uterine tissues of the early pregnant sheep were significantly higher than those of non-pregnant sheep (p0.05).Treatment of endometrial epithelial cells with WNT7A increased the mRNA expressions of β-catenin,c-myc and Cyclin D1.These results provided an underlying mechanism of periimplantation ovine conceptus development under induction of oestrus.     

不同剂量伊曲康唑制剂对犬血常规及肝肾功能的影响

旨在评价不同剂量伊曲康唑-环糊精制剂通过皮下注射途径对健康比格犬肝肾功能及血常规的影响.选用体重±10 kg的健康纯种比格犬32只,按试验要求随机分为4组,每组8只,建立稳定的生活制度.分别按照0.25 mg/kg、0.75 mg/kg和1.25 mg/kg剂量,皮下注射伊曲康唑制剂,3日1次,连续7次,对照组注射生理...