用绵羊小肠液冻干粉测定饲料过瘤胃淀粉小肠消化率方法的研究

本试验旨在以玉米为样本筛选用绵羊小肠液冻干粉测定精饲料瘤胃非降解残渣淀粉小肠消化率的最佳培养条件。分别研究了小肠液冻干粉用量(0.2、0.3、0.4、0.5和0.6g)对16h玉米瘤胃非降解残渣干物质和淀粉小肠消化率的影响;离体培养时间(4、8、12、16、20和24h)对16h玉米瘤胃非降解残渣干物质和淀粉小肠消化率的影响。结果表明,在本试验条件下,绵羊小肠液冻干粉测定玉米瘤胃非降解残渣淀粉小肠消化率的最佳用量为0.45g小肠液冻干粉/0.56g玉米瘤胃非降解残渣,最佳培养时间为12h。利用绵羊小肠液冻干粉测定常用饲料过瘤胃残渣淀粉小肠消化率的方法是可行的。     

半胱胺对中华鳖生长性能和非特异性免疫功能的影响研究

试验研究了半胱胺对中华鳖生长性能和非特异性免疫功能的影响,并对其机理进行了初步探讨。选取750只健康、活泼的中华鳖,平均体重(220±10)g,分成5个组,每个组设3个重复,每个重复50只。对照组基础日粮中不添加半胱胺,其余各组为试验组,半胱胺添加方式及添加量如下:试验Ⅰ组断续添加(每6天添加一次,6000mg/kg);试验Ⅱ组、试验Ⅲ组、试验Ⅳ组分别每天连续添加500、1000和1500mg/kg。试验期90d。试验结果表明:半胱胺能够提高中华鳖成活率、增重率、摄食率和饲料效率,且连续添加效果好于断续添加,当半胱胺含量达到1000mg/kg时,中华鳖增重率、摄食率和饲料效率达到最高(P<0.05);半胱胺使中华鳖血清胃泌素水平升高,血清生长抑素水平降低;1000mg/kg半胱胺可以显著提高中华鳖肌肉RNA/DNA比率(P<0.05);半胱胺还可以增强中华鳖血清谷胱甘肽过氧化物酶、超氧化物歧化酶活性,但不同添加方式及剂量之间无显著性差异,血清溶菌酶含量在500mg/kg半胱胺添加组最高(P<0.05)。由本试验结果可以看出,半胱胺对中华鳖具有促进生长、增强免疫的作用,是一种良好的生物添加剂,且其适宜添加量为每天连续添加1000mg/kg。     

蝴蝶兰花芽诱导过程中碳水化合物在叶与腋芽中的分配变化

 研究了粉色蝴蝶兰（KM 833）在两个不同条件下处理（处理组：人工气候箱日/夜温25℃/20℃；对照组：温室大棚生长条件）过程中叶片和腋芽中碳水化合物在叶与腋芽中的分配变化。结果发现对照的蝴蝶兰新叶开始时面积增长较快，但最后的叶面积的大小基本相同，处理组的单位叶面积干样质量在15 d后超过对照组；处理组蝴蝶兰叶片还原糖含量在20 d达到1个小高峰后下降，在30 d后开始急剧上升,至50 d达到最大值(31.08 mg·g^-1DM)，对照组的蝴蝶兰叶片还原糖含量在整个试验期间则较为恒定且缓慢地增长，腋芽中的还原糖含量则随时间而下降；两种处理蝴蝶兰叶片的可溶性糖和淀粉含量均随着时间的进程而逐步升高，处理组的蝴蝶兰腋芽中的可溶性糖和淀粉含量则在处理15 d内有个快速增加后缓慢下降，对照组腋芽的三类碳水化合物在处理期间处于上升趋势。无论在叶还是腋芽中,诱导组的碳水化合物含量均高于对照组。     

遮光对青榨械光合速率及叶绿素荧光参数的影响

研究了遮光15％、35％、50％和全光照处理对青榨槭新梢生长、叶片色素含量、净光合速率以及叶绿素荧光参数的影响。结果表明，随着遮光度增加，叶片色素含量增加，叶绿素a／b减小；叶片净光合速率（Pn）、初始荧光（Fo）、原初光能转化效率（Fv／Fm）和光化学猝灭系数（qP）增加，但非光化学猝灭系数（qN）降低。全光照和遮光15％处理条件下，Pn日变化呈双峰曲线，而35％和50％处理条件下呈单峰曲线；遮光35％和50％处理条件下Fv／Fm日变化幅度较小，15％和全光照处理条件下Fv／Fm日变化呈先上升后下降再上升趋势。50％遮光处理青榨槭幼苗Pn最高，新梢年生长量最大，可在育苗生产中应用。     

Mechanisms for protection of berberine against LPS-induced acute lung injury in mice

AIM:To investigate the mechanisms by which berberine attenuates LPS-induced acute lung injury, and provide a new strategy for the treatment of the lung injury due to LPS. METHODS:BALB/c mice were randomly assigned into three groups (control, LPS group, and berberine treatment group). Mice were administered intragastrically with distilled water (0.1 mL/10 g) or neutral sulfate berberine (50 mg/kg) once a day for 3 days, 1 h after intragastrical treatment on day 3, LPS (20 mg/kg) or normal saline was injected intraperitoneally (ip). All animals were sacrificed 12 h after LPS injection, the left lung tissue sections were prepared for histology analysis and the right lung were used to determine the ratio of wet to dry lung tissue weight (W/D). In another experiment, bronchoalveolar lavage fluid (BALF) was collected, and then the total protein content, and the amounts of white blood cells (WBC) and polymorphonuclear neutrophils (PMN) in BALF were determined. Furthermore, the phosphorylation of cytosolic phospholipase A₂ (cPLA₂) was detected with immunohistochemical analysis by using phospho-cPLA2(Ser505) antibody, and the contents of thromboxane B₂ (TXB₂) in BALF, malondialdehyde (MDA) in the lungs, and activity of superoxide dismutase (SOD) in lung tissues were also determined.RESULTS:LPS induced acute lung injury, activated cPLA₂, and increased TXB₂ content in the BALF and MDA level in the lung tissue. The pretreatment with berberine significantly attenuated lung injury, lung edema and protein leakage induced by intraperitoneal injection of LPS. The expression of phospho-cPLA₂ in the lung tissues and TXB₂ content in the BALF in the berberine treatment group were lower than those in LPS group (P<0.05). In addition, the content of MDA in the lung tissue was lower in the berberine treatment group than LPS group (P<0.05), but there was no significant difference in activity of lung SOD between the berberine treatment and LPS group (P>0.05). CONCLUSION:Pretreatment with berberine remarkably reduces the LPS-induced lung injury, which is, at least in part, through inhibiting phosphorylation of cPLA₂ and decreasing lipid peroxidation. These findings provide a new strategy for the prevention and treatment of LPS-induced acute lung injury.     

Myocardial dysfunction resulting from coronary microembolization

Coronary microembolization is a significant and frequent complication of primary percutaneous coronary intervention in the patients with acute myocardial infarction. More importantly, coronary microembolization is a main reason of dysfunction of microcirculation. The mechanism of myocardial disfunction resulting from coronary microembolition was associated with the vascular active materials released from platelet, platelet aggregation, which aggravate microembolization in microcirculation, endothelial dysfunction and inflammation.     

Activity of H+-K+-ATPase in gastric parietal cells under stress in rats and analysis of electron microscopic enzyme cytochemistry

AIM: To demonstrate the changes of activity and electron microscopic enzyme cytochemistry staining of H⁺-K⁺-ATPase of gastric parietal cells under stress in rats. METHODS: Twenty-four male SD rats were randomly divided into normal group, stress group and stress+omeprazole (OM) group. Water immersion-restraint stress (WRS) model in SD rats was performed. The ulcer index (UI) of gastric mucosa and H⁺-K⁺-ATPase activity of gastric parietal cells were measured. The changes of ultrastructure and electron microscopic enzyme cytochemistry staining of parietal cells were observed under transmission electron microscope (TEM). RESULTS: Compared with control group, the UI of gastric mucosa and H⁺-K⁺-ATPase activity of gastric parietal cells increased (P<0.01 and P<0.05) in stress group. In stress+OM group, both UI and H⁺-K⁺-ATPase activity decreased (P<0.01) compared with stress group. Parietal cells were in a resting state in control group, and became active in stress group, where plenty of intracellular canaliculi were observed under the TEM. In stress+OM group, the dilated intracellular canaliculi lined with rare microvilli were founded. Enzyme cytochemistry staining showed that there was little black punctate enzyme reactive product scatted in intracellular canaliculi and the apical plasma membrane of parietal cells in control group, and there were large amounts of black enzyme reactive product accumulated at the intracellular canaliculi in stress group. Scarcely deposition of enzyme reactive product in intracellular canaliculi was observed in stress+OM group. CONCLUSION: The results indicate that the H⁺-K⁺-ATPase activity of gastric parietal cells increases under WRS, and is in accordance with ultrastructure changes. These findings suggeste that gastric acid might be one of the most important factors that result in stress ulcer.     

Antiproliferation effects of 188Re labeled monoclonal antibody on prostate cancer cells in vitro

AIM: To investigate the effect of 188Re labeled monoclonal antibody on prostatic specific membrane antigen 7E11C5.3,radioimmunotherapy for the treatment of human prostate cancer cell line LNCaP in vitro.METHODS: 188Re-7E11C5.3 was prepared by direct 2-mercaptoethanol reduction method.Labeling efficiency and radiochemical purity was measured by paper chromatography.Immunoreactive fraction was determined by linear extrapolation.Cytotoxicity to LNCaP cells was determined by MTT assay.RESULTS: The labeling yield of 188Re-7E11C5.3 was (93.16±2.18)%,the radiochemical purity was (95.62±0.48)%,and the immunoreactive fraction was (74.86±1.86)%.The inhibitory effect of 188Re-7E11C5.3 on cell proliferation of LNCaP cells was significantly higher than that of 188Re-mIgG or 188ReO-4.The 50% inhibitory doses (IC50) of 188Re-7E11C5.3,188Re-mIgG,and 188ReO-4 were (23.38±3.73)×107 Bq/L,(59.21±8.02)×107 Bq/L and (68.89±10.91)×107 Bq/L,respectively.CONCLUSION: 188Re-7E11C5.3 can effectively inhibit the growth of in vitro cultured prostate cancer cells and shows much potential for prostate cancer radioimmunotherapy.     

不同果袋类型对紫花杧的套袋效果

以主栽品种紫花杧为试材,探讨不同果袋类型的套袋效果.结果表明:套袋可大幅度降低采收果的果面流胶和雨水污染,极显著地降低果面虫伤率.套袋可改变采收时的果面颜色,但不同果袋类型间存在差异.后熟完成时,果面均为品种固有颜色,不因果袋种类而改变.套袋能促进果实后熟转黄和果色均匀,能显著降低炭疽病的病果率,但不同果袋对蒂腐病的防效存在较大差异.套袋能提高可溶性固形物含量和减轻果实失重.供试品种用外黄内黑复合纸袋套袋效果最为理想.