猪肾脏中氯丙嗪和异丙嗪残留检测方法的建立

建立了猪肾脏中氯丙嗪和异丙嗪残留量检测的高效液相色谱法。猪肾脏中残留的氯丙嗪和异丙嗪,用乙腈提取,再依次用酸化乙腈和正己烷净化,氮气吹干,甲醇溶解后,用Waters高效液相色谱系统,HypersilC18柱,UV检测器,用V(乙腈)∶V(水)∶V(0.5mol·L-1乙酸铵)(50∶49∶1)为流动相,流速1.2mL/min,波长254nm测定,内标法定量。结果表明,氯丙嗪和异丙嗪在猪肾脏中的最低检测限均为10μg/kg,组织中添加量为10μg/kg时,氯丙嗪和异丙嗪的回收率分别为83%和84%,批间变异系数均小于20%。该方法样品处理简单,可同时检测氯丙嗪和异丙嗪在猪肾脏中的残留量。     

茄子组织培养再生体系研究初报

以茄子的子叶和下胚轴为外植体,研究了不同激素组合对外植体分化的影响,建立茄子下胚轴高效再生体系,并初步探讨了温度对植株再分化的影响.结果表明:下胚轴不定芽诱导的最适培养基为MS NAA 0.2 mg/L 6-BA 2.5 mg/L,芽诱导率为46%;子叶不定芽诱导的最适培养基为MS NAA 0.2 mg/L KT 2.0 mg/L,芽诱导率为37%.     

Pubertal development of male African catfish,Clarias gariepinus. In vitro steroidogenesis by testis and interrenal tissue and plasma levels of sexual steroids

In fish, sex steroids initiate and/or accelerate the maturation of the brain-pituitary-gonad axis. In order to obtain information on the steroid milieu during the pubertal development of male African catfish, we have monitored the conversion of [³H]-pregnenolone and [³H]-androstenedione by testis and [³H]-pregnenolone by interrenal tissue fragmentsin vitro. Pubertal development occurs between two and six months of age. Testicular development proceeds through four main stages that are characterised histologically by the presence of spermatogonia (stage I), spermatogonia and spermatocytes (stage II), spermatogonia, spermatocytes and spermatids (stage III), and all germ cells including spermatozoa (stage IV). 11β-Hydroxyandrostenedione and cortisol were the main products of testes and interrenal tissue, respectively, in all stages of the pubertal development; a change in the steroidogenic pattern was not observed during this period. The interrenal tissue displayed no significant conversion of [³H]-pregnenolone to 11-oxygenated androgens. Blood plasma was analyzed for the presence of five androgens; testosterone, 11β-hydroxytestosterone, 11β-hydroxyandrostenedione, androstenetrione, and 11-ketotestosterone. 11-Ketotestosterone was the quantitatively dominating androgen in the circulation at all stages of development, which was more pronounced in stages III and IV. The obvious differences between thein vitro andin vivo results, namely 11β-hydroxyandrostenedione being the main testicular productvs. 11-ketotestosterone dominating in the blood, may indicate that 11β-hydroxyandrostenedione is converted to 11-ketotestosterone at extratesticular sites.     

鲁西黄牛耳缘组织成纤维细胞的体外培养

实验以鲁西黄牛耳缘组织为研究材料,采用组织块贴壁培养法对其进行了成纤维细胞的体外培养。通过细胞的传代培养、形态学和动力学观察与分析,结果表明,所建立的鲁西黄牛耳缘组织成纤维细胞系具有典型的成纤维细胞形态,胞体均为梭形和不规则三角形,且细胞丰满;细胞核形态为卵圆形,并位于胞质中央,核仁清晰。在细胞生长于繁殖过程中亦经历了潜伏期、指数增生、停滞期和衰退死亡期等4个时期。细胞群体倍增时期为72h。实验结果表明,已成功地培养了鲁西黄牛耳缘组织成纤维细胞。     

草鱼ghrelin基因的分子克隆与组织分布及其摄食调控作用分析

ghrelin是一种在脊椎动物摄食调节过程中起重要作用的脑肠肽,具有明显的摄食促进作用。实验利用同源克隆技术获得了草鱼ghrelin基因的cDNA序列和DNA序列,其中cDNA序列全长506 bp,包括90 bp的5′端非编码区(5′-untranslated region,5′UTR),312 bp的开放阅读框(open reading frame,ORF),以及104 bp的3′端非编码区(3′-untranslated region,3′UTR)。开放阅读框编码的103个氨基酸的ghrelin前体肽,经剪切加工后形成含有19个氨基酸的成熟肽。氨基酸序列分析结果显示,草鱼ghrelin与硬骨鱼类ghrelin相似度最高,而与其他脊椎动物相似度较低,同时草鱼ghrelin成熟肽N端的"活性中心"(active core)为鲤科鱼类中常见的GTSF形式。与大多数硬骨鱼类的ghrelin基因结构相同,草鱼ghrelin基因也包括4个外显子和3个内含子。荧光定量PCR检测到ghrelin mRNA大量分布于草鱼的前肠和脾,脑、肾、肝、肌肉、皮和鳔等组织也有ghrelin mRNA分布。草鱼脑和肠中的ghrelin表达水平在摄食后下降,随着饥饿时间的延长表达水平逐步升高,最后维持在较高水平,表明ghrelin作为摄食启动信号对草鱼的摄食活动起到了促进作用。     

地被菊幼嫩花瓣组织培养研究

以地被菊幼嫩花瓣为试材,进行了组织培养的研究,结果表明地被菊幼嫩花瓣是诱导愈伤组织的良好材料。当培养基中2.4-D和NAA浓度为0.5～2mg·L-1时,愈伤组织诱导率均达87.2%以上,并且诱导出的愈伤组织结构疏松,易于分割。在分化培养基MS+KT2mg·L-1+IAA0.5mg·L-1上,芽分化率可达92.5%。不同接种方向对地被菊花瓣不定芽形成无显著影响。地被菊花瓣培养芽的分化率以基部组织为最高(94%),中部和上部组织分化率则逐渐变低。经培养得到的再生植株与原品种相比在形态上产生了一系列变化。     

异育银鲫体内阿维菌素血脑屏障渗透性及组织残留

采用脑组织匀浆法和高效液相色谱法(HPLC), 检测异育银鲫(Carassius auratus gibelio)体内不同浓度下阿维菌素(Avermectin, AVM)血脑屏障渗透性及其组织残留情况。结果显示, AVM在其3个半数致死浓度(24 h LC₅₀: 0.127 mg/L、48 h LC₅₀: 0.071 mg/L、96 h LC₅₀: 0.039 mg/L)及其安全用药浓度(0.003 9 mg/L)下, 均能从异育银鲫脑组织中检测出AVM; 其中24 h LC₅₀浓度下脑中AVM含量最高, 为(0.292±0.005) μg/g; 并且各半数致死浓度之间脑中AVM含量差异均极显著(P<0.05)。结果表明, 不同浓度条件下AVM均能渗透通过血脑屏障进入异育银鲫脑组织, 其含量与AVM用药浓度呈正相关。另外, 在安全用药浓度(0.003 9 mg/L)条件下, AVM在各组织中的浓度−时间数据经DAS 3.0药物代谢动力学软件拟合后发现均符合非房室模型, 其主要药代动力学参数大小关系表现为: (1)达峰时间(T_max): 肌肉<脑<肝<肾; (2)峰浓度(C_max): 肝>肾>肌肉>脑; (3)末端消除半衰期(T_1/2Z): 肝>脑>肾>肌肉; (4)药时曲线下面积(AUC): 肝>肾>脑>肌肉。本研究结果可为研究鱼类血脑屏障、AVM神经毒性及其在水产养殖上的应用提供参考。

     

大黄鱼冷诱导结合蛋白(CIRP)基因cDNA克隆及低温胁迫对其时空表达的影响

为研究冷诱导结合蛋白(CIRP)在大黄鱼低温适应过程中的作用,采用同源克隆技术获得了大黄鱼CIRP基因,并通过实时荧光定量PCR(qRT-PCR)技术检测了低温胁迫下大黄鱼各组织中CIRP基因的表达变化。结果显示,大黄鱼CIRP基因cDNA序列全长1211 bp,推测编码一个由182个氨基酸组成、分子量为19 ku的蛋白。序列比对显示硬骨鱼类CIRP基因序列较为保守,特别是N端的RNA识别基序(RRM)高度保守。系统进化树分析显示大黄鱼CIRP与银鳕相似性最高(81.5%),所有硬骨鱼类聚为一个大支。慢性低温胁迫中(12℃缓降至6℃),皮肤和肌肉中CIRP基因的表达量呈随温度降低而升高的趋势,6℃时表达量分别为12℃时的11.56倍和9.03倍;鳃、脑和心脏中CIRP基因表达量均呈先显著上升后显著下降的趋势,其峰值均出现在8℃时,表达量分别为12℃时的5.07、7.69和2.83倍;肠、肾脏、肝脏和脾脏中的表达量随温度降低而下降,6℃时的表达量最低,与12℃时相比降幅分别为80.0%、65.6%、91.2%、55.6%。急性低温胁迫(由12℃骤降至8℃并胁迫4 h)条件下,鳃、皮肤、脑、肝脏、心脏中CIRP基因表达量均呈先升高后降低的变化,反映了机体对低温胁迫的应激、适应过程;肌肉和肠中的表达量则始终显著低于胁迫前。慢性和急性低温胁迫中各组织CIRP表达量变化的差异提示,大黄鱼机体在低温胁迫响应和适应中有着多种调节机制。研究表明,CIRP基因参与了大黄鱼应对低温胁迫的过程。     

The effects of diet supplemented with Lactobacillus rhamnosus on tissue parameters of rainbow trout,Oncorhynchus mykiss (Walbaum)

This study was carried out to establish the effects of a 6 week treatment with the diet supplemented with L. rhamnosus in concentrations of 10⁷ CFU g^?1 (G1 group) and 10⁸ CFU g^?1 (G2 group) on the condition expressed by condition factors (Fulton's, Clark's and B), intestinal microbiology, haematological, histological and selected antioxidative parameters of rainbow trout. A significantly higher condition factors were found in G1 group indicating that higher concentration of probiotic (10⁸ CFU g^?1) did not result in the better condition. Cholesterol and urea levels were significantly higher in both G1 and G2 groups, albumin in G1 and creatinine in G2 group with respect to control. A significantly higher liver TBARS level was observed in G2 group. The feeding with supplemented probiont apparently changed the resident microbiota. Three weeks after withdrawal of the supplemented feed, the microflora mostly reverted to the control composition, although L. rhamnosus in faecal matter of fish remained inherent. The epithelial structure of the proximal and distal intestine revealed the increased absorptive area in both treated groups, as well as the increase in the mucin‐secreting goblet cells. The L. rhamnosus‐treated groups demonstrated the capacity for the augmentation of the innate host defence.     

奶山羊CIDEa基因的克隆、序列分析与组织表达

为获得奶山羊CIDEa基因序列并检测其在乳腺组织中的表达,采用RT-PCR技术从奶山羊乳腺组织扩增CIDEa基因序列,利用生物信息学软件对其进行预测分析,并采用荧光定量PCR检测CIDEa在干奶期和不同泌乳时期乳腺组织中的表达。结果表明:通过克隆测序得到奶山羊CIDEa基因CDS区660 bp,编码219个氨基酸,与GenBank公布的绵羊、牛、人和猪的核苷酸序列同源性分别为99%、96%、85%、85%。奶山羊CIDEa蛋白属于碱性、不稳定亲水蛋白,不存在跨膜结构和信号肽;蛋白主要定位在细胞质、线粒体和细胞核。CIDEa蛋白结构主要由α螺旋、β折叠和不规则卷曲组成。奶山羊CIDEa在泌乳前期、盛期和中期乳腺组织中表达量均显著高于干奶期(P<0.05)。说明CIDEa可能参与奶山羊乳腺的泌乳过程,为进一步研究其在奶山羊乳腺组织中的功能及对乳品质的调控作用奠定基础。