单端孢霉烯族毒素生物脱毒技术研究进展     

朱晓慧  陆启荣  胡嗣祎  王旭 《动物医学进展》2021,42(5):108-113

单端孢霉烯族毒素在粮食和饲料中污染严重,主要是T-2毒素和脱氧雪腐镰刀烯醇(DON)等,其毒性作用强,对人和动物产生严重危害。因此,单端孢霉烯族毒素的脱毒方式逐渐成为研究热点,尤其是生物脱毒。很多微生物被证实能够降解霉菌毒素,包括细菌、真菌和酵母菌,可将毒素降解成低毒或无毒的产物。论文以生物脱毒为出发点,从细菌、真菌和酵母菌三个角度概述了单端孢霉烯族毒素中T-2毒素和DON的脱毒研究现状,以期为后续开发并挖掘更加安全高效的生物脱毒方式提供参考。  相似文献   

1株降解黄曲霉毒素B1的解淀粉芽胞杆菌的分离鉴定及其体外脱毒效果     

张晓静  张杨杨  张晓峰  乔宏兴  边传周 《畜牧兽医学报》2021,52(8):2291-2301

旨在筛选出能够高效降解黄曲霉毒素B₁（AFB₁）的菌株,并对其脱毒活性组分的脱毒效果进行研究,本研究以香豆素为唯一碳源对目标细菌进行初筛,以对AFB₁的降解率为指标进行复筛,并从形态学、生理生化试验和16S rDNA序列分析对筛选菌株进行鉴定;通过测定该菌株不同发酵组分对AFB₁的降解率,来定位其脱毒活性组分,同时采用CCK-8法测定活性组分降解AFB₁后对LMH细胞毒性,并研究了热处理、紫外线照射、强酸、强碱及蛋白酶K处理对活性组分脱毒作用的影响。结果显示,从样品中初筛分离到24株能够在初筛培养基生长良好的菌株,经复筛从中筛选到一株能高效降解AFB₁的菌株Y1-B1,其AFB₁降解率达到73.2%;经形态学、生理生化试验和16S rDNA序列分析确定该菌为解淀粉芽胞杆菌（Bacillus amyloliquefaciens）。对菌株Y1-B1培养物的不同组分进行的脱毒活性研究表明,不同组分对AFB₁的降解率不同,上清液的脱毒能力最强,细菌细胞裂解物的脱毒能力下降明显,菌体悬液和菌体裂解物上清的脱毒能力最差,由此确定解淀粉芽胞杆菌Y1-B1的脱毒能力主要来源于上清液中的某种活性物质;细胞毒性结果显示,与AFB₁对LMH细胞的毒性作用相比,AFB₁被上清液降解后其产物的毒性显著降低。该脱毒活性组分对不同理化因素处理呈现出不同的表现,对高温、紫外照射抵抗力较强,对强酸、强碱抵抗力较差,蛋白酶K仅造成脱毒能力部分减弱。本研究将为解决黄曲霉毒素污染问题提供新的微生物种质资源,同时为后续微生物脱毒制剂的开发奠定基础。  相似文献   

植物病毒及脱毒研究之进展     

刘娜 《北京农业》2012,(21):80-81

植物病毒是一个极小的微粒.近几十年来,有关植物病毒的研究已取得很大的进展,对某些作物病毒的症状、寄生范围、传播途径、病理现象、鉴定方法及无毒苗培育途径等均已进行了深入的研究.  相似文献   

瘤胃微生物对饲料中霉菌毒素的脱毒作用     

龙淼  李鹏  张燚  朱连勤  刘国文  王哲 《中国饲料》2012,(1):37-39,43

反刍动物瘤胃内微生物数量巨大、种类繁多,具有多种生理功能,对霉菌毒素也具有高效的脱毒作用。本文介绍了近年来瘤胃微生物对几种主要的霉菌毒素的脱毒作用。  相似文献   

菜籽饼中硫葡萄糖甙的去除方法     

张振红  黄仁录  马可为 《中国饲料》2006,(17):42-43

硫葡萄糖甙(GS)是菜籽饼中主要的抗营养因子。本文对硫葡萄糖甙的性质及其降解产物的毒害作用和菜籽饼的脱毒方法进行综述。  相似文献   

棉蚜对吡虫啉抗性的初步研究   总被引：1，自引：1，他引：1       下载免费PDF全文

李菁  韩召军 《农药学学报》2007,9(3):257-262

用吡虫啉对棉蚜进行室内抗性筛选,用药处理25次后抗性是筛选前的20.03倍;2007年对田间棉蚜进行抗性调查,发现不同地区种群对吡虫啉的抗性差异显著,江苏南京种群最为敏感,河南安阳、山东泰安和北京地区棉蚜与之相比,抗性分别为2.21、7.63和9.53倍;抗、感品系解毒酶活力分析发现,抗性品系的谷胱甘肽S-转移酶活性增加很少(比活力1.12倍),但酯酶活力显著高于敏感品系(比活力1.71倍);增效试验结果表明,顺丁烯二酸二乙酯(DEM)在抗、感品系中对吡虫啉均没有明显的增效作用,而磷酸三苯酯(TPP)和增效醚(PBO)虽然在敏感品系中对吡虫啉的增效作用较小(SR 1.24和1.29),但在抗性品系中的增效作用显著增高(SR 2.13和1.74);此外还发现,吡虫啉处理可提高棉蚜群体的酯酶活力。由此认为,棉蚜至少具有对吡虫啉产生中等水平抗性的风险,其抗性可能是由于棉蚜的酯酶和P450单加氧酶的解毒能力提高所致。  相似文献   

Pisatin demethylation by fungal pathogens and nonpathogens of pea: association with pisatin tolerance and virulence     

L. M. DELSERONE  K. McCLUSKEY  D. E. MATTHEWS  H. D. VANETTEN   《Physiological and Molecular Plant Pathology》1999,55(6):317

Previous studies have indicated that detoxification of their hosts' phytoalexins is a tolerance mechanism for some true fungi, but not the fungus-like Oomycota, and may be involved in determining the virulence of a pathogen. In the present study, the associations between demethylation of the pea phytoalexin pisatin, tolerance to pisatin, and virulence on pea were examined for 50 fungal isolates which represent 17 species of pathogens and nonpathogens of pea. All isolates ofPythium coloratum and P. irregulare failed to metabolize and were sensitive to pisatin, consistent with previous observations that members of the Oomycota generally lack the ability to metabolize and are sensitive to their hosts' phytoalexins. Among true fungi tested, the ability to demethylate pisatin was common, regardless of whether the particular isolate was pathogenic on pea or not. However, when the rate of pisatin demethylation was compared to virulence, all but one of the moderate to highly virulent isolates rapidly demethylated pisatin. In addition, the more rapidly demethylating isolates were generally more tolerant of pisatin. These results suggest that a specialized enzyme system for quickly detoxifying pisatin might be present in most pea pathogens. In previous studies a specific cytochrome P450 enzyme for demethylating pisatin was identified in the pea pathogen Nectria haematococca mating population VI, and genes (PDA genes) encoding that enzyme have been cloned from this fungus. When DNA specific for these genes was used to probe genomic DNA from other fungi that demethylate pisatin, significant hybridization was detected with only one fungus, the pea pathogen Fusarium oxysporum f. sp. pisi. If the other pea pathogens possess a specific cytochrome P450 system for detoxification of pisatin, the genes encoding these enzymes apparently share limited nucleotide similarity with N. haematococca PDA genes.  相似文献   

4株Ⅰ亚群禽腺病毒分离株对SPF雏鸡的致病性研究     

谢梓民  曾繁聪  傅禹铭  姜含雨  杨惠湖  柯骏鸿  罗瑞  梁昭平  张雪莲  黄淑坚 《中国畜牧兽医》2022,49(3):1032-1040

【目的】 探究Ⅰ亚群禽腺病毒（Fowl adenovirus,FAdV）分离株GDDL-4（FAdV-4）、GDB3-8a （FAdV-8a）、GDT08-8b （FAdV-8b）、GDWYT-11（FAdV-11）对SPF雏鸡的致病性,进而制定更加有效的防控措施。【方法】 设立4个攻毒组（GDDL-4、GDB3-8a、GDT08-8b、GDWYT-11）及对照组,攻毒组选择腿部肌内注射接种0.2 mL 10⁵ TCID₅₀病毒液,对照组接种等体积PBS。接种后观察SPF雏鸡的临床症状、剖检病变及组织病理学变化,同时检测其排毒量和病毒载量。【结果】 所有攻毒组鸡均表现为精神沉郁、消瘦、扎堆等,病理剖检以严重心包积液-包涵体肝炎综合征病变为主,其中GDDL-4组症状最为严重,死亡率最高达85%,总体死亡率在0~85%之间。排毒分析结果发现,GDDL-4和GDB3-8a组出现高滴度排毒（≥10⁴拷贝/μL）,GDT08-8b和GDWYT-11组仅能检测到低滴度（≤10³拷贝/μL）排毒。器官指数表明,除GDT08-8b组与对照组无明显差异外,其余攻毒组均能造成器官不同程度的肿大或萎缩。病理组织学切片显示,肝脏、肾脏、法氏囊的正常结构被破坏,可见肝细胞有大量淋巴细胞浸润、肾间质充血出血、法氏囊淋巴细胞坏死等。病毒载量分析结果显示,GDDL-4与GDWYT-11组在肝脏组织中病毒滴度最高,而GDB3-8a与GDT08-8b组在十二指肠中病毒滴度最高。【结论】 Ⅰ亚群FAdV的死亡率高,4株分离株均可导致雏鸡肝脏出现包涵体肝炎的病理变化,均可反复排毒,且分离株对不同的组织器官有不同的亲嗜性,在肝脏与十二指肠等组织中的病毒载量最高。  相似文献   

速康解毒口服溶液对兔皮肤刺激性和过敏性的实验研究     

黄鑫  郝宝成  高旭东  刘建枝  王保海  梁剑平 《中国草食动物》2015,35(1)

试验旨在为评价动物疯草中毒解毒治疗药物——速康解毒口服溶液的临床前应用安全性,为临床推广应用提供实验依据.用速康解毒口服溶液、赋形剂(蒸馏水)局部涂抹大白兔破损皮肤及完整皮肤,并逐日观察症状表现,统计观察结果.用速康解毒口服溶液或赋形剂、2,4-二硝基氯苯(DNCB)对大白兔多次致敏,并于2周后观察大白兔的反应.结果表明:速康解毒口服溶液对家兔完整皮肤刺激反应的平均分值为零,属于无刺激药物,对破损皮肤也无明显刺激;在过敏性实验中,给药组5只家兔中1只有轻微的过敏现象,结合致敏反应评价的分值法和致敏反应发生率,速康解毒口服溶液对家兔皮肤过敏反应的分值为0.2(1/5),致敏率为20％(1/5),具有弱致敏性.结论:速康解毒口服溶液对家兔皮肤无明显刺激性,有轻微过敏现象,属于临床安全药物.  相似文献   

Gene expression in pyriproxyfen-resistant Bemisia tabaci Q biotype     

Ghanim M  Kontsedalov S 《Pest management science》2007,63(8):776-783

Pyriproxyfen is a biorational insecticide that acts as a juvenile hormone (JH) analogue and disrupts insect development with an unknown molecular mode of action. Pyriproxyfen is one of the major insecticides used to control the whitefly Bemisia tabaci (Gennadius) and comply with integrated pest management (IPM) programmes, resulting in minimal effects on the environment, humans and beneficial organisms. During the last few years, resistance to pyriproxyfen has been observed in several locations in Israel, sometimes reaching a thousandfold or more. No information exists about the molecular basis underlying this resistance that may lead to understanding the mode of action of pyriproxyfen and developing molecular markers for rapid monitoring of resistance outbreaks. In this communication, a cDNA microarray from B. tabaci was used to monitor changes in gene expression in a resistant B. tabaci population. Based on statistical analysis, 111 expressed sequence tags (ESTs) were identified that were differentially upregulated in the resistant strain after pyriproxyfen treatment. Many of the upregulated ESTs observed in the present study belong to families usually associated with resistance and xenobiotic detoxification such as mitochondrial genes, P450s and oxidative stress, genes associated with protein, lipid and carbohydrate metabolism and others related to JH-associated processes in insects such as oocyte and egg development.  相似文献