脲酶抑制剂与硝化抑制剂对稻田土壤氮素转化的影响

【目的】本研究旨在阐明脲酶抑制剂(urease inhibitor,UI)和硝化抑制剂(nitrification inhibitor,NI)对稻田土壤氮素转化的影响,探讨抑制剂提高稻谷产量以及氮肥利用率的机理。【方法】本试验设在我国南方红壤稻田,共5个处理:1)不施氮肥(CK);2)尿素(U);3)尿素+脲酶抑制剂(U+UI);4)尿素+硝化抑制剂(U+NI);5)尿素+脲酶抑制剂+硝化抑制剂(U+UI+NI);脲酶抑制剂采用N-丁基硫代磷酰三胺(NBPT),硝化抑制剂采用3,4-二甲基吡唑磷酸盐(DMPP)。在水稻分蘖期和孕穗期测定土壤脲酶活性、硝酸还原酶活性、土壤铵态氮含量、硝态氮含量以及微生物碳、氮的含量,分析NBPT与DMPP对水稻两个主要生育期土壤氮素供应的影响,比较各处理的产量以及氮肥利用率,通过逐步回归分析研究以上各指标对产量的影响,探明脲酶抑制剂NBPT与硝化抑制剂DMPP在稻田的增效机理。【结果】1)与单施尿素相比,添加NBPT以及NBPT与DMPP配施均显著提高稻谷产量与地上部氮素回收率,两个处理分别增产6.56%与8.24%,氮素回收率提高幅度为19.4%与23.7%。2)与单施尿素相比,添加NBPT以及NBPT与DMPP配施,显著降低水稻分蘖期的土壤脲酶活性和铵态氮含量,显著提高孕穗期的铵态氮含量,而对此时期的脲酶活性无显著影响,所有处理对两个时期的硝态氮含量、硝酸还原酶活性、微生物量碳、氮含量均无显著影响;因此,NBPT对于抑制脲酶活性以及提高铵态氮含量的作用主要在孕穗期之前,而单施DMPP没有显著效应。3)从各项土壤指标与水稻产量相关性的逐步回归分析结果来看,水稻分蘖期与孕穗期稻田土壤中铵态氮含量对水稻产量影响显著,而且孕穗期的影响大于分蘖期,其余指标则对产量无显著影响。【结论】脲酶抑制剂NBPT以及NBPT与硝化抑制剂DMPP配施显著提高孕穗期土壤中的铵态氮含量,显著提高稻谷产量以及地上部氮素回收率,证明了生产上氮肥后移的重要意义。     

赤霉素及机械处理的相互作用对破除Sandersonia aurantiaca种子休眠的研究

在预备试验的基础上，选用了21种促进种子发芽的方法，结果显示，完整的s．aurantiaca种子对任何处理都无响应，砂纸磨擦 近胚根处切除小部分可使种子发芽率提高至11％。以上处理结合300mg／L GA3溶液的使用可破除种子休眠，使种子发芽率提高到69％以上。结果还表明，S．aurantiaca种子发芽的适宜温度为20℃；25℃ 16h／d光照及30℃的条件可降低种子的发芽率。研究还对S．aurantiaca种子的吸胀能力以及所含抑制物对生菜种子发芽的影响进行了比较。初步得出，S．aurantiaca种子具有种皮限制和种胚休眠的双重休眠机制，GA3和机械处理的相互作用可破除种子休眠。     

绢丝昆虫茧丝蛋白酶抑制剂含量的比较分析

以 6种绢丝昆虫的茧壳为材料 ,对茧丝蛋白酶抑制剂的含量及热稳定性进行了研究。结果表明 :家蚕品种间茧丝蛋白酶抑制剂的含量差异极显著 ,外层丝中含量较多 ,F1代的含量呈双亲中间型 ,偏向于含量较多的亲本 ,雌雄间含量无显著差异 ;家蚕茧丝蛋白酶抑制剂对热稳定性较强 ;天蚕绿茧、野蚕的茧丝中有少量的蛋白酶抑制剂存在 ,蓖麻蚕的茧丝中有微量蛋白酶抑制剂存在 ,天蚕黄茧、柞蚕茧、樗蚕茧的茧丝中基本无蛋白酶抑制剂存在。     

Development and characterization of monoclonal antibodies against canine trypsin

Canine cationic trypsin was purified by salting-out, gel filtration and affinity chromatography. Purity was confirmed by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE). The molecular weight was ca. 28 kDa by SDS-PAGE.

Thirty hybridomas were obtained which produced mAb to canine cationic trypsin by the cell fusion technique. Twenty-two of these recognized cationic trypsin only, while eight hybridomas recognized both cationic and anionic trypsin. Several of the anti-canine cationic trypsin mAb were purified by salting-out and DEAE ion-change chromatography using ascites fluid of immunized BALB/c mice. The mAb proved to have very high specificity to canine cationic trypsin as shown by immunoblotting and it may be possible to use them to develop clinical assays.     

组氨醇脱氢酶抑制剂的研究动态

组氨醇脱氢酶(HDH)是组氨酸生物合成过程中最后两步反应的催化酶。对组氨醇脱氢酶的结构、催化机理、组氨醇脱氢酶抑制剂等方面的研究动态进行了较为详细的综述。     

Gly-Gly肽和Gly-L-Leu肽在蛋鸡肠道内水解的研究

采用蛋鸡离体外翻肠段培养法,将小肠分为十二指肠、空肠前段、中段、后段和回肠五个部位肠段,洗净外翻。2种二肽培养液(Gly-Gly肽和Gly-L-Leu肽溶液)作为两组对照培养液,每种二肽培养液中添加肽酶抑制剂(Bestatin和Amastatin),作为试验培养液,39.5℃培养25min,每5min取样一次,测定培养液中的二肽含量。结果表明,培养5min后,含Gly-Gly肽的对照和试验培养液中均未能检测到完整Gly-Gly肽。而含Gly-L-Leu肽的对照培养液Gly-L-Leu肽的含量降低到16.75％,试验培养液则下降到43.40％。而试验培养液中Gly-L-Leu肽的含量10min后无显著降低(P>0.05)。各培养时段试验培养液Gly-L-Leu含量均显著高于对照培养液(P<0.05)。由此认为,离体肠囊在培养过程中能够迅速释放肠肽酶及一些生物活性物质,快速水解2种二肽。肽酶抑制剂(Bestatin和Amastatin)能抑制Gly-L-Leu的水解,但不能抑制Gly-Gly的水解。     

几种脲酶抑制剂对大豆脲酶和绵羊瘤胃微生物脲酶的抑制作用

本文研究了脲酶抑制剂乙酰氧肟酸 (AHA)、邻苯二酚、氢醌 (HQ)和硼砂对大豆脲酶和绵羊瘤胃微生物脲酶的抑制作用。结果表明 ,在浓度为 0 .0 0 0 1,0 .0 0 1,0 .0 1和 0 .1mmol/L时 ,4种脲酶抑制剂对大豆脲酶的抑制率分别为 :AHA为 6 % ,6 .2 % ,9.6 6 %和 2 9.79% ;HQ为 8.4 % ,13.0 3% ,19.79%和 4 4 .75 % ;邻苯二酚为 2 0 .34% ,19.12 % ,83.16 %和 93.78% ;而硼砂为 16 .5 5 % ,17.18% ,18.95 %和 35 .5 0 %。在相同浓度下 ,4种脲酶抑制剂对绵羊瘤胃微生物脲酶的抑制率分别为 :AHA为 9.5 8% ,14 .0 4 % ,4 1.30 %和 72 .73% ;HQ为 12 .2 1% ,39.99% ,6 4 .6 2 %和 78.87% ;邻苯二酚为 6 .0 7% ,9.36 % ,31.2 9%和 5 0 .4 4 % ;而硼砂分别为 4 .97% ,8.6 3% ,2 1.78%和 32 .0 2 %。     

Treatment of canine haemangiosarcoma with suberoylanilide hydroxamic acid, a histone deacetylase inhibitor

A case report is presented by describing the treatment of a 12‐year‐old dog – diagnosed with haemangiosarcoma (HSA) – with suberoylanilide hydroxamic acid (SAHA), a histone deacetylase (HDAC) inhibitor. The drug was administered orally, on a daily basis, approximately 2 weeks post‐splenectomy at a dose of 3 mg kg^?1. HSA is a lethal malignancy of the endothelium, which is usually disseminated by the time it is diagnosed. Median survival time, usually, is no longer than 80 days. Following treatment with SAHA, no sign of malignant growth could be discerned by means of diagnostic abdominal ultrasound, chest X‐ray or with the help of clinical symptoms, over a period of >1000 days. The precise mechanism by which HDAC inhibitors exert their anti‐cancer effects is uncertain, but evidence suggests that exposure to SAHA generates hyperacetylated chromosomal histones, which, in turn, facilitates the expression of tumour suppressor genes turned off by epigenetic mechanisms during neoplastic transformation of the endothelium.     

Non-target toxicology of a new mosquito larvicide, trypsin modulating oostatic factor

Trypsin modulating oostatic factor (TMOF), a peptide hormone originally isolated from the ovaries of adult Aedes aegypti, is currently under commercial development as a new pesticide chemistry with a novel mode of action for the control of larval mosquitoes. The objective of the current research is to evaluate potential risks of the use of TMOF as an insecticide on non-target organisms. TMOF (YDPAP₆) was degraded in vitro (as determined by HPLC and LC/MS) to DPAP₆, PAP₆, and then AP₆ by leucine aminopeptidase, a pancreatic enzyme found in the digestive system of vertebrates. The rate of degradation of TMOF and PAP₆ was significantly greater than that of DPAP₆, while no metabolism of AP₆ was found. TMOF technical insecticide was produced on a commercial scale by recombinant yeast (heat-killed before application). The technical TMOF when administered in a single dose by gavage to male and female mice at 2000 mg dry weight/kg body weight produced no negative effects as compared to controls up to 12 days after treatment. When male and female mallard ducks were treated by gavage with 1250 mg dry weight of technical TMOF/kg body weight each day for 5 days, again no toxic effects were noted through 35 days after the last treatment. TMOF technical insecticide was also applied to the shaved skin of male and female rabbits at the rate of 2000 mg/kg for 1-2 days, with no effect. The end point observations in these in vivo experiments were mortality; changes in growth rate, behavior, body structure, and color; and possible lesions observed during necropsy. Finally, Daphnia incubated with technical TMOF in rearing water at the level of 1.0 × 10⁶ yeast cells/ml (10 mg/ml) also demonstrated no negative effects on mortality, growth, molting, time to first brood, and production of viable neonates. It appears from these studies that TMOF can be degraded by vertebrate digestive proteases and technical TMOF is not toxic to the non-target organisms examined.     

Effect of benazepril and pimobendan on serum angiotensin‐converting enzyme activity in dogs

To support their combined use, the objective of the study was to evaluate the effects of benazepril and pimobendan on serum angiotensin‐converting enzyme (ACE) activity in dogs. A total of 48 healthy beagle dogs were randomized into four groups (n = 12 per group) in a parallel‐group design study: A (control, placebo twice daily (BID)); B (0.5–1.0 mg/kg benazepril once daily (SID) in the morning, placebo in the evening); C (0.25–0.5 mg/kg benazepril BID); D (0.25–0.5 mg/kg benazepril and 0.125–0.25 mg/kg pimobendan, both BID). The test items were administered orally for 15 days. Serum ACE activity was measured on days 1 and 15. Groups B, C and D had significantly lower average serum ACE activity compared to baseline and to the control group, on both days 1 and 15. There were no significant differences in average ACE activity between groups B, C and D. Noninferiority of group C to B was demonstrated. In conclusion, 0.25–0.5 mg/kg benazepril administered BID produced noninferior inhibition of serum ACE activity compared to 0.5–1.0 mg/kg benazepril dosed SID. Pimobendan had no significant effect on benazepril's action on serum ACE activity. The results support the use of benazepril BID in dogs and in combination with pimobendan.