桃红四物汤口服合清热解毒利湿方溻渍治疗下肢丹毒的临床研究

目的观察桃红四物汤口服合清热解毒利湿方溻渍对下肢丹毒的疗效与作用。方法以随机数字表法将62例下肢丹毒患者分为对照组(31例,37患侧)和观察组(31例,38患侧)。对照组采用常规治疗(抗生素静滴+硫酸镁溶液外敷+抬高患肢休息),观察组在上述疗法的基础上予以桃红四物汤口服+清热解毒利湿方溻渍。对比两组青霉素使用率和使用量,治疗前后红肿面积,临床疗效,治疗前后血白细胞计数(WBC)、中性粒细胞百分比(N%)、血清C反应蛋白(CRP)水平,不良反应和复发率。结果两组青霉素使用率和使用量对比差异均无统计学意义(P>0.05);两组治疗后红肿面积均缩小,且治疗后观察组红肿面积小于对照组,上述差异均有统计学意义(P<0.05);两组临床疗效总有效率差异均有统计学意义(P<0.05),且观察组总有效率高于对照组(P<0.05);治疗后两组血WBC、N%、血清CRP水平均下降(P<0.05),且观察组均低于对照组(P<0.05);两组不良反应发生率和6个月内复发率差异均无统计学意义(P>0.05)。结论桃红四物汤口服合清热解毒利湿方溻渍治疗下肢丹毒可缩小红肿面积,增强疗效,减轻炎症反应,且安全,远期疗效好。

化瘀解毒方提取物抑制作用胃癌细胞增殖和黏附及对PI3K/Akt通路影响的实验研究

目的:研究化瘀解毒方提取物抗胃癌细胞增殖和黏附方面的作用及机制。方法:采用高效液相色谱法(HPLC)分析化瘀解毒方提取物稳定性,化瘀解毒方提取物作用于人胃癌SGC-7901细胞株,利用MTT分析细胞增殖抑制实验,检测红细胞毒性实验,MTT快速测定法测定活性峰与Matrigel的黏附作用的影响。Western blot法检测人胃癌SGC-7901细胞中PI3K,PDK1和Akt总蛋白及其磷酸化水平的影响。结果:化瘀解毒方提取物可浓度依赖性抑制体外人胃癌SGC-7901细胞增殖、黏附,免疫印迹结果显示,化瘀解毒方提取物抑制Akt蛋白磷酸化,然而对于上游蛋白PDK1和PI3K的磷酸化无作用。结论:化瘀解毒方提取物抑制其增殖和黏附,其作用机制可能与抑制PI3K/Akt通路有关。

黄连解毒汤70%醇提物对小鼠S_(180)细胞MDR相关因子表达的逆转作用

目的观察黄连解毒汤70%醇提物对小鼠多药耐药(MDR)基因表达产物P170、肺耐药蛋白(LRP)和拓扑异构酶(TOPO)的影响,明确其干预MDR的分子生物学基础,指导临床应用其逆转MDR的产生。方法模拟临床PFC方案,建立小鼠S180肿瘤细胞MDR在体模型,同时给予黄连解毒汤70%醇提物10d,流式细胞仪荧光检测P170、LRP、TOPO。结果黄连解毒汤70%醇提物明显逆转S180肿瘤细胞MDR相关基因表达产物P170、LRP、TOPO的过度表达。结论黄连解毒汤70%醇提物可通过逆转相关生物活性物质的过度表达,逆转化疗诱发的肿瘤MDR的产生。

黄连解毒汤醇提物预防给药对MDR模型小鼠相关基因表达产物的影响

目的:观察黄连解毒汤70%醇提物预防给药对小鼠多药耐药(MDR)基因表达产物P170、肺耐药蛋白(LRP)和拓扑异构酶Ⅱ(TOPOⅡ)的影响,探讨其干预MDR的分子生物学基础,指导临床应用以预防MDR的产生。方法:小鼠随机分为非耐药模型组、耐药模型组、黄连解毒汤70%醇提物100,50mg·kg^(-1)组,模拟临床PFC方案,建立小鼠S180肿瘤细胞多药耐药在体模型,同时给予黄连解毒汤70%醇提物4周,流式细胞仪荧光检测P170,LRP,TOPOII。结果:黄连解毒汤70%醇提物明显降低化疗诱导后耐药细胞P170,LRP的表达率和ROPOII活性。结论:黄连解毒汤70%醇提物可通过对相关生物活性物质的调节,干预和逆转化疗诱发的肿瘤MDR的产生。

黄连解毒汤70%醇提物对MDR模型小鼠细胞凋亡及相关因子表达的影响

目的:观察黄连解毒汤70%醇提物对MDR模型小鼠S180肿瘤细胞P170、细胞凋亡及其相关细胞因子的影响,进一步探讨其干预肿瘤细胞多药耐药的分子生物学基础,指导临床应用。方法:建立小鼠S180肿瘤细胞多药耐药在体模型,同时给予黄连解毒汤70%醇提物4 w,流式细胞荧光检测P170、Fas、CD54及细胞凋亡。结果:黄连解毒汤70%醇提物可显著增加凋亡基因Fas表达率、耐药肿瘤细胞凋亡率并降低细胞黏附因子CD54的表达。结论:黄连解毒汤70%醇提物可通过对相关生物活性物质的调节,干预和逆转化疗诱发的肿瘤细胞多药耐药的产生。

氰化物解毒药的研究——4-二甲胺基苯酚及4-氨基苯丙酮衍生物的合成

合成了4-二甲胺基苯酚(1)及4-氨基苯丙酮(2)的衍生物23个,并经过氰化钠(12μg/g,sc)中毒小鼠筛选,发现化合物4c、7a 和9a,b 抗氰化钠中毒有效,其中化合物9b 效果明显优于化合物2。

黄连解毒汤有效成分的提取及其对体内白色念珠菌的清除作用

试验旨在研究黄连解毒汤有效成分的提取及对其体内白色念珠菌的清除作用。分别采用水煎煮和乙醇回流提取法,随后乙醇提取物用3种不同极性的有机溶剂萃取(正丁醇、乙酸乙酯、石油醚),以最小抑菌浓度为指标优化出最佳抑菌效果的提取工艺;观察给药前后系统性感染白色念珠菌小鼠肾脏、肝脏的真菌负荷量及活性氧(ROS)含量水平的变化,并检测血清中细胞因子白细胞介素-6(IL-6)、IL-1β、白细胞介素-1β前体(pro-IL-1β)及肿瘤坏死因子-α(TNF-α)的含量。结果显示,黄连解毒汤抑菌效果最优的提取工艺为:料液比1∶30,乙醇浓度60%,温度80℃,提取时间1 h,提取次数2次,测得乙酸乙酯萃取物MIC 90为0.3125 mg/mL。与模型组相比,黄连解毒汤乙酸乙酯提取物(EAHD)高剂量组能显著降低小鼠肾脏真菌负荷量(P<0.05),完全治愈率达40%,并明显高于氟康唑组;EAHD低、中和高剂量组(50、100及200 mg/(kg·d))均能显著降低肝脏真菌负荷量(P<0.05),其中中剂量组和氟康唑组降低肝脏真菌负荷量效果接近。同时EAHD高剂量组能显著或极显著降低感染后小鼠肾脏和肝脏ROS含量(P<0.05;P<0.01);显著或极显著提高血清中IL-6、IL-1β和TNF-α的含量(P<0.05;P<0.01),同时降低pro-IL-1β含量。综上所述,通过优化后的提取工艺得到的EAHD具有降低模型小鼠肾脏和肝脏ROS含量和调控炎症因子的作用,进而降低炎症反应,起到保护组织和抵抗白色念珠菌的作用。

对苯二酚与杂交中DNA的相互作用

目的探讨在pH为7.42磷酸盐缓冲溶液中对苯二酚与DNA的相互作用。方法用循环伏安法、荧光光谱法、紫外光谱法、DNA分子杂交技术和量子化学方法进行检测。结果在DNA杂交过程中,对苯二酚与其作用后的荧光光谱,紫外光谱的吸收峰峰形以及强度改变较大,循环伏安法氧化峰正向移动,量化计算结果表明,对苯二酚位于磷酸基团和碱基近侧。结论在DNA杂交过程中对苯二酚与其以∏-∏化学键和静电结合为主。

短评:百草枯中毒怎样做血液净化?

关于治疗急性百草枯中毒（paraquatpoosoning，PQP）方面，虽然血液透析（HD）、连续性血液净化（CRRT）、血液灌流（HP）以及血浆置换等方法分别有成功救治的报道，尤其是HP的成功资料最为突出。但是否具备循证医学证据，还有待更多临床资料的积累和分析。这些年，我们不断地摸索PQP的各种治疗方法，我个人认为，治疗PQP的三大基石是血液净化、免疫抑制剂的应用和及早排除毒物的有效措施。但是无论采用什么方法，成功救治率一直徘徊在50％～60％。血液净化清除血液中的毒物，首先要了解毒物的毒代动力学。而我们对百草枯的毒代动力学的理解基本来源于动物实验，或者是根据已有的临床资料进行的推测，并未完全搞清楚。

黄连解毒汤乙酸乙酯提取物抑制白念珠菌菌丝的形成

目的:探讨黄连解毒汤乙酸乙酯提取物(ethyl acetate extract of Huanglian Jiedu decoction,EAHD)对白念珠菌菌丝形成的影响。方法:以0,78,312,1 250 mg·L-1EAHD干预白念珠菌6 h,采用倒置显微镜、荧光显微镜及扫描电镜分别观察白念珠菌菌丝形态;固体培养基上观测菌落形态;实时荧光定量PCR(qRT-PCR)检测白念珠菌菌丝形成相关基因HWP1,ALS3,UME6,SUN41,CSH1,Ca PDE2的表达量。结果:312,1 250 mg·L-1EAHD可显著抑制白念珠菌菌丝的形成及菌落的形态;qRT-PCR检测显示1 250 mg·L-1EAHD使HWP1,ALS3,UME6,CSH1表达分别下调4.13,3.64,2.46,2.75倍,SUN41表达上调7.26倍,Ca PDE2表达无变化。结论:EAHD可能通过抑制HWP1,ALS3,UME6,CSH1等相关基因的表达来抑制白念珠菌菌丝的形成。

黄连解毒汤乙酸乙酯提取物对白假丝酵母菌黏附作用的影响

目的探讨黄连解毒汤乙酸乙酯提取物(ethyl acetate extract of Huanglianjiedu decoction,EAHD)对白假丝酵母菌黏附作用的影响。方法 XTT法检测白假丝酵母菌黏附力;平板法计数导管上黏附的白假丝酵母菌CFU;倒置显微镜观察黏附的白假丝酵母菌;qRT-PCR法定量检测黏附相关基因EAP1、HWP1、ALS1、ALS3、MP65的表达。结果 312μg/mL EDHA可显著抑制白假丝酵母菌在聚苯乙烯和聚酯导管上的黏附;白假丝酵母菌生长早期在EDHA作用下,菌细胞出芽数均呈现剂量依赖性降低;EDHA作用后,EAP1、HWP1均下调,ALS3、MP65均上调,ALS1几乎未变化。结论 EAHD可显著抑制白假丝酵母菌的黏附作用。

黄连解毒汤70%醇提物对MDR模型小鼠S180肿瘤细胞凋亡因子表达的影响

目的:观察黄连解毒汤70%醇提物对MDR模型小鼠S180肉瘤细胞凋亡因子的影响,探讨其逆转多药耐药作用的分子机制。方法:模拟临床PFC方案,建立小鼠S180肉瘤细胞多药耐药在体模型,同时给予黄连解毒汤70%醇提物灌胃10d,流式细胞仪荧光检测观察细胞凋亡因子Fas、Trail、细胞黏附因子CD54等指标。结果:黄连解毒汤70%醇提物增加耐药细胞凋亡因子Fas、Trail表达率,促进耐药S180细胞的凋亡,降低细胞黏附因子CD54的表达。结论:黄连解毒汤70%醇提物促进耐药细胞凋亡因子的高表达,是其逆转肿瘤多药耐药的途径之一。

Cumulative Toxicity of Residue Degradation Products of Penicillin Bacteria

[Objective] The research aimed to discuss the accumulation of toxic slag of penicillin bacteria residue degradation products and explore its ability to meet the aquaculture industry as a protein feed into development and utilization conditions.[Method] Through the sub-acute toxicity tests in mice strains,which were fed by different doses of penicillin bacteria residue degradation products （3% and 6%） under continuous observation of 15 weeks,recording a weekly mouse weight and death,and sampling executed after the test,animal liver and kidney function were blood test,taking heart,liver,spleen,kidney weighing,as well as liver and kidney pathology observed in the optical microscope.[Result] There were no significant differences （P 0.05） between the test group mice body weight,mortality and liver and kidney function and the control group within 15 weeks.Low-dose test group could be seen the liver cells,renal tubular epithelial nuclei broken,and a small number of liver and kidney cells with mild edema.High-dose test group could be seen in liver tissue of mice nuclei fragmentation and a fat droplets,the majority of liver cells,edema,and only a small number of liver cells,there were no significant changes.Renal portal area showed inflammatory cell infiltration,renal tubular epithelial cells,edema and necrosis.[Conclusion] In this experimental condition,the degradation products of penicillin bacteria residue played a mild toxcity on organ parenchymal cells in mice.

黄连解毒汤乙酸乙酯提取物对光滑念珠菌黏附作用的影响

目的:探讨黄连解毒汤乙酸乙酯提取物(ethyl acetate extract of Huanglian Jiedu decoction,EAHD)对光滑念珠菌Candida glabrata黏附作用的影响。方法:采用二倍稀释法测定黄连解毒汤乙酸乙酯提取物对光滑念珠菌的最低抑菌浓度(minimum inhibitory concentration,MIC);采用XTT还原法评价EAHD对光滑念珠菌黏附作用的影响;利用倒置显微镜、扫描电子显微镜与荧光显微镜观察EAHD对光滑念珠菌早期黏附形态学影响;采用半定量与实时荧光定量PCR检测其黏附相关基因EPA1,EPA6和EPA7的表达量。结果:EAHD对光滑念珠菌的MIC为320 mg·L-1,阳性对照药氟康唑对光滑念珠菌的MIC为1 mg·L-1;EAHD对光滑念珠菌2,4 h的黏附的干预作用较明显,其中对4 h效果优于2 h;PCR结果显示EAHD可显著抑制EPA1,EPA6和EPA7的表达。结论:EAHD可能通过抑制光滑念珠菌部分黏附基因的表达而抑制其早期黏附。

浮选锑尾矿回收金的试验研究

青海某锑金矿选矿厂采用"先锑后金"的优先浮选流程,因矿石氧化程度高,泥化现象严重,导致浮选金精矿品位及回收率很低。为了提高金的选矿回收率,对选锑尾矿采用CIL提金试验研究,金浸出率为65.10%,相比较原选矿工艺金回收率提高52.95%。

Advances in Biodegradation of Aflatoxins

Aflatoxins are secondary metabolites of fungi such as Aspergillus flavus and Aspergillus parasiticus. They are one of the contaminants most common in food and feed, with high toxicity and carcinogenicity. Aflatoxins usually enter animal body together with feed and then enter human body by food chain, thereby seriously threatening human health. In recent years, the degradation of aflatoxins has become a hot research topic. This study overviewed the characteristics and detoxification ways of aflatoxins, specifically for the advances in biodegradation and degradation products of aflatoxins.

化痰通瘀解毒方水提取物通过Wnt/β-catenin信号通路抑制人胃癌细胞株MKN-45上皮-间质转化及侵袭迁移

目的:观察化痰通瘀解毒方对人胃癌细胞MKN-45侵袭迁移能力和上皮-间质转化(Epithelial-mesenchymal transformation,EMT)的影响,并探讨其与Wnt/β-catenin信号通路的相关性。方法:以转化生长因子-β1(Transforming growth factor-β1,TGF-β1) 10 ng/m L诱导MKN-45细胞构建EMT模型;采用Transwell小室实验和划痕愈合实验检测细胞的侵袭、迁移能力;采用Western Blot法检测EMT标志蛋白E-cadherin、N-cadherin、Vimentin、Snail和Wnt/β-catenin信号通路相关蛋白表达水平。结果:TGF-β1能够明显增强MKN-45细胞侵袭、迁移能力,诱导MKN-45细胞发生EMT:E-cadherin蛋白表达下调,N-cadherin、Vimentin和Snail蛋白表达上调;同时,TGF-β1能诱导MKN-45细胞Wnt1和β-catenin蛋白表达上调。化痰通瘀解毒方(10、20、40μg/m L)均可显著抑制TGF-β1诱导的MKN-45细胞侵袭迁移及EMT:E-cadherin蛋白表达上调,N-cadherin、Vimentin和Snail蛋白表达下调;同时,化痰通瘀解毒方(10、20、40μg/m L)还可下调Wnt1和β-catenin蛋白表达,且上述结果中化痰通瘀解毒方在10、20、40μg/m L剂量组间存在剂量依赖性; Wnt/β-catenin信号通路特异性抑制剂XAV939与化痰通瘀解毒方40μg/m L均可明显抑制TGF-β1诱导的MKN-45细胞EMT和侵袭迁移,且XAV939可协同化痰通瘀解毒方40μg/m L抑制TGF-β1诱导的EMT和侵袭迁移。结论:化痰通瘀解毒方能通过Wnt/β-catenin信号通路抑制TGF-β1诱导的EMT,进而降低MKN-45细胞侵袭迁移能力。

Chromium detoxification mechanism induced growth and antioxidant responses in vetiver(Chrysopogon zizanioides(L.) Roberty)

This study investigated the chromium(Cr)detoxification mechanism-induced changes in growth and antioxidant defence enzyme activities in Chrysopogon zizanioides.Plant growth decreased by 36.8%and 45.0%in the shoots and roots,respectively,in the 50 mg/L Cr treatment.Cr accumulation was higher in root(9807μg/g DW)than in shoots(8730μg/g DW).Photosynthetic pigments and malondialdehyde content increased up to the 30 mg/L Cr treatment,whereas they declined at higher doses.The activity of superoxide dismutase(SOD),catalase(CAT)and peroxidase(POX)were increased significantly with increasing of Cr dose but slightly declined at higher doses.Isozyme banding patterns revealed the expression of multiple bands for SOD,CAT and POX enzymes,and the band intensity decreased at high doses of Cr exposure.These results indicate that higher Cr doses increased the oxidative stress by over production of reactive oxygen species(ROS)in vetiver that had potential tolerance mechanism to Cr as evidenced by enhanced level of antioxidative enzymes,photosynthetic pigments,MDA contents.Therefore,vetiver has evolved a mechanism for detoxification and accumulates higher concentration of toxic Cr.This study provides a better understanding of how vetiver detoxifies Cr.

Comparison of Detoxification Methods on Phorbol Esters in Deoiled Jatropha curcas Meal for Animal Feeds

The deoiled Jatropha curcas meal by hexane extraction was detoxified phorbol esters by two different methods. These two methods were alkali in methanol and only ethanol washing. After both treatments, the PEs （phorbol esters） was decreased by 100%. The crude protein in detoxified meal of alkali in methanol washing was less amount than only ethanol washing. The result showed that treatment by only ethanol washing was a promising way to detoxify deoiled Jatropha curcas meal for animal feeds in industrial scale.

Biodegradation of microcystin-RR and -LR by an indigenous bacterial strain MC-LTH11 isolated from Lake Taihu

The indigenous bacterial strain MC-LTH11 with the capability of degrading microcystin-RR MC-RR and microcystin-LR MC-LR was successfully isolated from Lake Taihu.The bacterium was identified as Stenotrophomonas sp. which possessed a mlrA gene. The MC-LTH11 thoroughly degraded MC-RR and MC-LR with the initial concentration of 37.13 mg/L and 18.49 mg /L respectively in the medium containing crude microcystins extract within 6 d.The degradation rates were affected by temperature pH initial MCs concentration and the kinds of media. Additionally the bacterial strain MC-LTH11 also degraded thoroughly microcystins in the water body of Lake Taihu within 1 d.These results suggest that the Stenotrophomonas sp.MC-LTH11 has the capacity to bioremediate water bodies contaminated by microcystins and may contribute to the degradation of microcystins after the outbreak of harmful cyanobacterial blooms in Lake Taihu.