眼镜蛇毒因子

摘要： 目的 探讨淫羊藿苷( ICA)对补体旁路激活造成的小鼠急性肺损伤的保护作用及作用机制.方法 32只昆明小鼠随机分为正常对照组、模型组、PDTC组、淫羊藿苷组,预防给药7d 后,用特异性补体旁路激活蛋白眼镜蛇毒因子(CVF),尾静脉注射复制小鼠急性肺损伤模型.测定小鼠支气管肺泡灌洗液( BALF)中蛋白含量和炎性细胞数目;肺组织匀浆后测定髓过氧化物酶( MPO)活性; ELISA 法检测BALF和血清中 IL-6、TNF-α、P-selectin、ICAM-1 的含量;HE染色法观察肺组织病理形态学变化;免疫组化法测定肺组织中NF-κB p65的磷酸化水平,并采用双萤光素酶报告基因检测系统,在细胞水平上测定补体旁路激活对微血管内皮细胞中NF-κB的核内转录活性的影响.结果 ICA可以明显降低小鼠肺组织匀浆液中 MPO 含量和 BALF 中炎性细胞数目,并同时降低BALF中IL-6、TNF-α、P-selectin含量和血清中TNF-α、P-selectin、ICAM-1 水平,减轻小鼠肺部炎性细胞浸润,明显抑制小鼠肺组织中NF-κB p65 的磷酸化,并有效抑制NF-κB核内转录活性的上调.结论 ICA能有效减轻补体旁路激活诱导的小鼠肺部急性炎症反应,其机制可能与抑制肺组织炎性细胞浸润、NF-κB p65的磷酸化及核内转录活性,从而降低炎症反应水平有关.%Aim To explore the protective effect and mechanism of icariin ( ICA ) on acute lung injury ( ALI) in mice induced by activation of the comple-ment alternative pathway. Methods 32 healthy KM mice were randomly divided into four groups: the nor-mal group, the model group, the PDTC group and the Icariin group, which received 7-day intragastric admin-istration respectively. Then cobra venom factor ( CVF) was used to activate specifically complement alternative pathway to induce acute lung injury in mice by intrave-nous injection. Myeloperoxidase ( MPO ) activity of lung homogenate, the cell count and the protein con- tent of bronchoalveolar lavage fluid ( BALF ) were measured. The concentration of IL-6, TNF-α, P-selec-tin and ICAM-1 in BALF and serum were determined by ELISA. The pathological change of lung tissue was observed by HE staining. The phosphorylation of NF-κB p65 in lung tissues was checked by immunohisto-chemistry. The effect of the transcriptional activity of NF-κB signal pathway in microvascular endothelial cells was measured by employing dual-luciferase re-porter assay system. Results ICA reduced MPO ac-tivity of lung homogenate, the cell count and the con-tent of IL-6, TNF-α, P-selectin in BALF obviously. The level of TNF-α, P-selectin and ICAM-1 in serum was decreased, the pulmonary inflammatory cell infil-tration was reduced, the phosphorylation of NF-κB p65 in lung was inhibited significantly and the transcrip-tional activity of NF-κB was also down-regulated. Con-clusion ICA can alleviate acute inflammatory re-sponse of ALI mice induced by activation of the com-plement alternative pathway. The mechanism may be highly related to the inhibition of inflammatory cell in-filtration in lung tissue, the down-regulation of phos-phorylation of NF-κB p65 and nuclear transcriptional activity.

摘要： 本文探讨了绿原酸对补体旁路激活致小鼠急性肺损伤的保护作用及可能的作用机制.将32只KM小鼠随机分为正常对照组、模型组、白藜芦醇组、绿原酸组,预防给药7d后,用特异性补体旁路激活蛋白眼镜蛇毒因子(CVF)尾静脉注射复制小鼠急性肺损伤模型.测定肺含水量、肺组织匀浆中髓过氧化物酶(MPO)活性、支气管肺泡灌洗液(BALF)中细胞数目和蛋白含量,ELISA法检测BALF和血清中白介素-6(IL-6)、肿瘤坏死因子(TNF-α)、P选择素(P-selectin)和细胞间黏附分子-1(ICAM-1)的含量,HE染色法观察肺组织病理形态学变化,免疫组化法测定肺组织中NF-κB p65的磷酸化水平.研究发现,绿原酸可以降低小鼠BALF中蛋白含量、炎性细胞数目、IL-6和TNF-α含量以及肺组织匀浆中MPO活性,并可显著降低血清中IL-6、TNF-α及P-selectin、ICAM-1水平;病理形态学显示绿原酸可以显著抑制炎性细胞浸润,免疫组化结果显示绿原酸可显著抑制小鼠NF-κB p65的磷酸化水平.以上结果说明绿原酸可明显减轻补体旁路激活诱导的小鼠急性肺损伤,其机制可能与抑制NF-κB p65的磷酸化及降低炎症反应程度有关.

摘要： 目的:观察眼镜蛇毒因子(cobra venom factor,CVF)对脓毒症大鼠外周血中肿瘤坏死因子-α(TNF-α)、白介素-6(IL-6)和白介素-10(IL-10)的影响.方法:选取清洁级雄性SD大鼠144只,按照随机数字表法将大鼠分为A组(假手术组)、B组(脓毒症组)、C组(CVF预处理组),各48只;各组按照标本采集点的不同又分为术后2、4、8、12、16、24 h六个时间点亚组,各8只.B、C组采用盲肠结扎穿孔术(CLP)制作脓毒症大鼠模型;C组大鼠在CLP术前静脉注射CVF,而A、B组静脉注射等量0.9％ 氯化钠溶液.观察术后大鼠一般情况及腹腔情况,比较各组术后不同时间点的TNF-α、IL-6和IL-10水平变化.结果:C组大鼠脓毒症反应较B组明显减轻;除术后8 h外,C组术后其他时间点TNF-α 水平均低于B组(P<0.05),其中B组术后2 h时TNF-α 迅速升高达峰然后下降,但是术后12 h再次升高出现第二个峰值,C组术后4 h较2 h迅速下降,术后8 h再次升高出现第二个峰值;除术后16 h外,C组术后其他时间IL-6水平均低于B组(P<0.01);除术后2、24 h外,C组血清IL-10水平均高于B组(P<0.05),而且术后8、16 h两次达到峰值,呈双峰变化.结论:CVF可以有效维持促炎细胞因子(TNF-α、IL-6)和抗炎细胞因子(IL-10)的平衡并明显抑制脓毒症大鼠的炎症反应,同时TNF-α 及IL-10的"双峰现象"也为免疫平衡理论及PICS提供了理论依据.

摘要： Aim To investigate the change of coagulation and fibrinolysis functions of human microvascular endothelial cells (HMEC) induced by activated complement alternative pathway and effect of pyrrolidine-dithiocarbamate (PDTC) and resveratrol (Res) on intervention.Methods Normal human serum was activated by cobra venom factor (CVF).After exposure of HMEC to activated complement for various time points, supernatant was removed and assayed for activities of hydrolysing chromogenic substrate and affecting activated partial thromboplastin time (APTT) and prothrombin time (PT).The cells exposed to activated complement were collected and washed, and then the cell suspension was assayed for activity of affecting coagulation function of normal plasma.Lastly, the coagulation and fibrinolysis functions of HMEC pretreated with PDTC and Res were also investigated after HMEC was exposed to activated complement alternative pathway.Results The hydrolysis activity of chromogenic substrate of supernatant was up-regulated significantly after HMEC exposed to activated complement alternative pathway.The supernatant induced APTT decreased significantly, and also shortened PT.The cell suspension of various time points induced APTT decreased significantly, and also shortened PT by suspension of 6 h time point.PDTC and Res failed to inhibit the up-regulation of the chromogenic hydrolysis activity, but Res showed significant intervention on decrease of APTT, and PDTC had better effect on inhibiting the decrease of PT than that of Res.Conclusion Activated complement alternative pathway can induce abnormality of coagulation and fibrinolysis functions of HMEC, and PDTC and Res can affect this change.%目的 研究补体旁路激活导致的微血管内皮细胞纤溶凝血功能的变化以及吡咯烷二硫氨基甲酸(PDTC)和白藜芦醇(Res)的干预作用.方法 采用眼镜蛇毒因子激活血清补体旁路途径.将补体旁路活化的血清作用于人微血管内皮细胞(HMEC),检测多个时间点细胞培养上清的水解发色底物活性变化和对凝血酶原时间(PT)、活化部分凝血活酶时间(APTT)的影响,并制备细胞悬液,检测细胞表面的抗凝血功能变化情况.采用PDTC、Res对上述变化指标进行干预研究.结果 HMEC经补体旁路活化产物刺激后,细胞培养上清的发色底物酶解活性明显上调;细胞培养上清导致正常血浆的APTT明显缩短,同时,对PT也有缩短的作用;经补体旁路活化产物刺激HMEC后制备的各时间点细胞悬液对正常血浆的APTT有明显的缩短作用,6 h刺激组的细胞悬液也表现出缩短PT的作用.PDTC和Res未能抑制发色水解活性的上调,但Res对APTT的缩短有明显的干预作用,而PDTC能在一定程度上抑制PT的缩短.结论 补体旁路活化产物会导致HMEC纤溶凝血功能的失调,而PDTC和Res有一定的干预作用.

摘要： 目的：研究补体旁路激活所导致的小鼠肺部急性炎症的发生发展及相关指标的变化,为药物筛选及干预研究提供理想的小鼠肺部急性炎症病理模型。方法 SPF级昆明小鼠尾静脉注射眼镜蛇毒因子( CVF)激活血清补体旁路途径,根据注射后取样时间不同,分为15 min、30 min、1 h、2 h、6 h组,同时平行设置PBS对照组。取肺组织测定肺系数、肺含水量,并行病理切片检查,肺组织匀浆测定髓过氧化物酶(MPO)活性；制备支气管肺泡灌洗液(BALF)和血清,测定BALF中的细胞数和蛋白含量,采用 ELISA 法分别测定BALF和血清中的 IL-6、TNF-α、P-selectin 和 ICAM-1含量。结果小鼠尾静脉注射 CVF后可致肺部炎性细胞明显浸润,MPO活性明显上调,BALF中细胞总数和蛋白浓度明显增加。 BALF和血清中的IL-6、TNF-α、P-selectin水平及血清中ICAM-1的含量均明显升高,其中,BALF中P-selectin含量在30 min时间点出现1个小高峰,IL-6和TNF-α在1 h时间点出现1个高峰,在2h时间点均无进一步上升,但在6h时间点各指标均又明显升高；血清中IL-6和TNF-α含量在1 h时间点达到峰值,随后浓度降低, P-selectin和ICAM-1水平随着时间的延长持续上升。而肺系数、肺含水量及BALF中ICAM-1的含量与PBS组相比无明显变化。结论补体旁路激活可导致小鼠肺部急性炎症的发生,以30 min至1 h的炎症反应最为明显,该实验可以为药物筛选及干预研究提供理想的动物肺部急性炎症病理模型。%Aim To study the development of acute lung inflammation in mice induced by activation of the complement alternative pathway and the changes of the related indicators, and to provide an ideal pathological model of acute lung inflammation in mice for drug screening and intervention. Methods Cobra venom factor( CVF) was used to activate complement alterna-tive pathway of SPF Kunming mice by intravenous injection. According to different sampling time, the mice were divided into 15 min, 30 min, 1 h, 2 h, 6 h group, and the parallel PBS control groups were set at the same time. Lung coefficient, lung water content, myeloperoxidase ( MPO ) activity, BALF cell number and protein content were tested. The pathological changes of lung tissue were observed by HE staining. The concentration of IL-6 , TNF-α, P-selectin and ICAM-1 in bronchoalveolar lavage fluid ( BALF ) and serum were determined by ELISA. Results CVF caused pulmonary inflammatory cell infiltration in mice obviously. Compared with PBS groups, MPO activity of lung tissue, BALF cell and the protein concentration were significantly increased. The contents of IL-6, TNF-α, P-selectin in BALF and serum were in-creased, and the content of ICAM-1 in serum was also increased. The content of P-selectin in BALF reached the first peak at 30 min point, the content of IL-6 and TNF-α in BALF reached the first peak at 1 h point, but the indicators had no further changes at 2 h point, and all the indicators rose again at 6 h point. The lev-els of IL-6 and TNF-α in serum reached peak at 1 h point,then the content showed lower levels at the sub-sequent time points. The levels of P-selectin and ICAM-1 in serum increased along the time. Lung coef-ficient, lung water content and ICAM-1 of the BALF showed no significant alteration. Conclusion The ac-tivation of the complement alternative pathway can lead to acute lung inflammation in mice and the inflammato-ry response is the most obvious at 30 min to 1 h. The study could provide an ideal pathological model of a-cute lung inflammation in mice for drug screening and intervention.

摘要： 目的：揭示流感病毒介导的小鼠肺部炎性损伤机制，为研发治疗病毒性肺炎的有效药物提供理论和技术依据。方法建立流感PR8感染小鼠动物模型，利用实时荧光定量PCR、ELISA、病理切片等方法检测小鼠肺部炎症因子、补体分子及病理变化；按照50μg／（kg·24 h）的剂量腹腔注射眼镜蛇毒因子（CVF），监测小鼠体质量、存活率、炎症因子等变化。结果与对照组相比，PR8流感模型组小鼠肺组织中补体调节分子Crry、CD59表达显著下降（P＜0．01），补体分子C9和补体成分受体C3aR、C5aR表达显著升高（P＜0．01），血清中促炎因子TNF-α、IL-6、IFN-γ高表达，抗炎因子IL-2低表达（P＜0．05）；经CVF药物干预后，小鼠体质量下降缓慢，存活率升高，肺指数降低（P＜0．05），抗炎因子IL-2表达明显升高（P＜0．05），促炎因子IL-6、TNF-α、INF-γ表达显著下降。结论补体激活参与了流感病毒介导的肺部炎性损伤；通过CVF干预，抑制了补体激活，可提高感染小鼠存活率，降低肺指数，延缓病程。%Objective To investigate the mechanism of pulmonary inflammation induced by influenza virus , and provide reference for the development of effective drugs for viral pneumonia .Methods An influenza PR8 infection mouse model was established .The levels of inflammatory cytokines and complement molecules were determined using RT -PCR and ELISA.The pathological changes were examined using biopsy .The complement inhibitor cobra venom factor ( CVF) was injected intraperitoneally at a dose of 50 μg/( kg· 24 h) , and then body mass .The survival rate and inflammatory factors were examined .Results Compared with the control group , the expressions of complement regulatory molecule Crry and CD59 were significantly decreased (P<0.01), while those of complement C9 and complement receptor C3aR and C5aR were significantly increased in the lungs of influenza model mice (P<0.01).Pro-inflammatory cytokines TNF-α, IL-6 and IFN-γwere highly expressed , but anti-inflammatory cytokine IL-2 was lowly expressed in serum .Treatment with CVF caused a sight body mass loss, a survival rate increase and a lung index decrease (P <0.05).Moreover, an IL-2 expression increase and a decrease of IL-6, TNF -αand INF-γexpression were observed in CVF treatment mice ( P< 0.05).Conclusion Inhibition of complement activation can increase the survival rate of mice with influenza pneumonia and decrease pulmonary indexes .thus delaying the pathogenesis of PR 8.

摘要： 目的 揭示流感病毒介导的小鼠肺部炎性损伤机制,为研发治疗病毒性肺炎的有效药物提供理论和技术依据。方法 建立流感PR8感染小鼠动物模型,利用实时荧光定量PCR、ELISA、病理切片等方法检测小鼠肺部炎症因子、补体分子及病理变化; 按照50μg/（kg·24 h）的剂量腹腔注射眼镜蛇毒因子（CVF）,监测小鼠体质量、存活率、炎症因子等变化。结果 与对照组相比,PR8流感模型组小鼠肺组织中补体调节分子Crry、CD59表达显著下降（P〈0.01）,补体分子C9和补体成分受体C3aR、C5aR表达显著升高（P〈0.01）,血清中促炎因子TNF-α、IL-6、IFN-γ高表达,抗炎因子IL-2低表达（P〈0.05）; 经CVF药物干预后,小鼠体质量下降缓慢,存活率升高,肺指数降低（P〈0.05）,抗炎因子IL-2表达明显升高（P〈0.05）,促炎因子IL-6、TNF-α、INF-γ表达显著下降。结论 补体激活参与了流感病毒介导的肺部炎性损伤; 通过CVF干预,抑制了补体激活,可提高感染小鼠存活率,降低肺指数,延缓病程。

摘要： Aim To investigate the effect of resveratrol ( Res) , PDTC and AG490 on adhesion molecules ex-pression induced by product of activated complement alternative pathway on human microvascular endothelial cells ( HMECs) and the possible mechanisms. Meth-ods HMECs were exposed to the product of comple-ment alternative pathway activation, then the superna-tant was removed to detect the concentration of malond-ialdehyde ( MDA ) with TBA method. ELISA method was used to detect the expression of soluble ICAM-1 , VCAM-1 ( and E-selectin) in the culture supernatant. Res, PDTC and AG490 with different concentrations were used to determine their effect on cell oxidation level and adhesion molecules expression. The phospho-rylation of NF-κB p65 was detected by Western blot, and the intervention of Res, PDTC and AG490 was as-sayed by the same way. Results The activation of complements alternative pathway resulted in the phos-phorylation of NF-κB p65 , and increased the concen-tration of MDA and up-regulated the expression of ICAM-1, VCAM-1 and E-selectin. Res reduced the concentration of MDA. Res, PDTC and AG490 inhibi-ted the phosphorylation of NF-κB p65 . Res and PDTC showed similar inhibition on expression of ICAM-1 and VCAM-1 , while exhibiting little effect on expression of E-selectin, and AG490 significantly inhibited the ex-pression of the above adhesion molecules. Conclusions Res, PDTC and AG490 could inhibit the expression of adhesion molecules induced by activated complement alternative pathway, the inhibition of NF-κB pathway activation was involved in their mechanism, and JAK2 may be a more important intervention target in regula-ting adhesion molecule expression.%目的：研究白藜芦醇( Res)、PDTC和AG4903种化学小分子对补体旁路激活致人微血管内皮细胞炎症反应相关黏附分子表达的干预作用和可能的作用机制。方法采用补体旁路激活产物作用于人微血管内皮细胞( HMEC )。TBA法检测细胞培养上清中丙二醛(MDA)的浓度,ELISA方法检测细胞培养上清中可溶性黏附分子ICAM-1、VCAM-1、E-selectin的表达,并采用多个浓度的Res、NF-κB信号通路抑制剂PDTC和JAK2信号通路抑制剂AG490预处理内皮细胞,研究3种抑制剂对细胞氧化水平和黏附分子表达的干预作用。利用Western blot检测补体旁路激活产物作用于内皮细胞对NF-κB p65磷酸化的影响及3种抑制剂的干预作用。结果 HMEC受补体旁路激活产物刺激后,导致细胞培养上清中MDA浓度升高, NF-κB p65磷酸化和黏附分子ICAM-1、VCAM-1和E-selectin的表达上调。 Res可降低细胞培养上清中MDA的浓度。 Res、PDTC和AG490能抑制NF-κB p65的磷酸化。 Res与PDTC能抑制内皮细胞黏附分子ICAM-1和VCAM-1的表达,对E-selectin的表达有一定的抑制作用,而AG490能够明显抑制上述3种黏附分子的表达。结论 Res、PDTC和AG490对补体旁路激活产物致内皮细胞黏附分子表达上调有不同程度的抑制作用,其作用机制与NF-κB信号通路的活化有关,而JAK2可能是一个更重要的调控位点。

摘要： 本发明公开了应用多克隆抗体亲和柱纯化眼镜蛇毒神经生长因子的方法，包括以下步骤：将眼镜蛇毒预处理后，通过NGF‑多克隆抗体亲和柱进行吸附、洗脱和进一步纯化，得到眼镜蛇毒神经生长因子；所述NGF‑多克隆抗体亲和柱为：通过眼镜蛇毒NGF基因原核表达，纯化分离得到重组眼镜蛇毒NGF；将重组眼镜蛇毒NGF作为免疫原，免疫动物得到抗血清，并分离纯化得到NGF多克隆抗体；将NGF多克隆抗体与载体结合交联所得。利用基因重组技术，使用产量较高的重组神经生长因子，激发动物产生能蛇毒NGF的多克隆抗体，进而规模化制备NGF‑多克隆抗体亲和柱，利用免疫亲和的特异性及高效性；对天然蛇毒神经生长因子纯化，得到天然的、高活性的蛇毒神经因子。减少生产成本，适应规模化生产。

摘要： 本发明公开了一种适于规模化生产的眼镜蛇蛇毒神经生长因子的纯化方法，是将冻干的眼镜蛇蛇毒溶解后用硫酸铵溶液进行沉淀，然后离心取上清液，采用截留分子量为3K的超滤膜膜包超滤，交换缓冲液至pH 5.0浓度为50mM的NaAc缓冲溶液，交换完缓冲液的样品上样于CM Sepharose FF柱层析，收集目的蛋白，上样于Superdex 75柱，收集目的蛋白，得到眼镜蛇蛇毒神经生长因子原液，本发明与现有技术方法相比提高了处理量和得率，适用于规模化生产。

摘要： 本发明公开了本发明涉及一种眼镜蛇毒神经生长因子的制备方法，将眼镜蛇粗毒进行两次凝胶层析，其中凝胶层析Ⅰ为SP‑Sephadex G‑25柱层析，凝胶层析Ⅱ为Acta Rosorse柱层析。本发明提供的眼镜蛇毒神经生长因子制备方法简单易行、可用于工业化放大生产、活性损失小，活性损失小于25％的蛇毒NGF；可以打破蛋白质分离的常规限制，使用更高初始浓度的粗蛇毒液也可以进行有效分离；生产效率高、成本合理，特别适合工业化规模生产；得率高，超过0.5％，甚至能达到0.6％以上。

摘要： 本发明公开了应用多克隆抗体亲和柱纯化眼镜蛇毒神经生长因子的方法，包括以下步骤：将眼镜蛇毒预处理后，通过NGF‑多克隆抗体亲和柱进行吸附、洗脱和进一步纯化，得到眼镜蛇毒神经生长因子；所述NGF‑多克隆抗体亲和柱为：通过眼镜蛇毒NGF基因原核表达，纯化分离得到重组眼镜蛇毒NGF；将重组眼镜蛇毒NGF作为免疫原，免疫动物得到抗血清，并分离纯化得到NGF多克隆抗体；将NGF多克隆抗体与载体结合交联所得。利用基因重组技术，使用产量较高的重组神经生长因子，激发动物产生能蛇毒NGF的多克隆抗体，进而规模化制备NGF‑多克隆抗体亲和柱，利用免疫亲和的特异性及高效性；对天然蛇毒神经生长因子纯化，得到天然的、高活性的蛇毒神经因子。减少生产成本，适应规模化生产。

摘要： 本发明公开了一种眼镜蛇毒神经生长因子纯化制备方法，先采用DEAE CL?6B阴离子交换柱然后再利用Sephadex G?50凝胶层析柱、Macro?prep High S阳离子交换柱依次进行分离，每次分离后采用PC12细胞检验法用超纯水对所收集的各峰稀释后进行检验选取蛇毒神经生长因子活性最高的峰作为下步分离的样品。其中，通过稀释测定NGF诱导PC12细胞分化的最小浓度，发明人找到了蛇毒分离过程中NGF的最高活性峰，并确定NGF诱导PC12细胞分化的最小浓度达到0.1μg/ml。试验表明，应用本发明可得到电泳纯的NGF，其纯度高、活性高。

摘要： 本发明涉及一种眼镜蛇毒神经生长因子将骨髓间充质干细胞诱导分化成软骨细胞的方法，它包括：从眼镜蛇毒中分离纯化NGF；从SD乳鼠的四肢骨髓中分离出间充质干细胞；将一定数目的干细胞悬液加入到含有NGF的培养基中进行诱导培养，诱导7、14、21天后，通过免疫组化、糖胺多糖定量检测以及聚合酶链式反应等技术手段研究自提取的蛇毒NGF对大鼠骨髓间充质干细胞的软骨诱导作用。实验结果表明眼镜蛇毒NGF能促进该细胞向软骨方向分化，说明眼镜蛇毒NGF是一种有潜力的治疗软骨缺损的生长因子，经本发明方法的诱导，所产生的软骨细胞可用于大规模的体内移植治疗软骨缺损，有利于软骨组织工程的临床推广和应用。

摘要： 本发明公开了眼镜蛇毒神经生长因子在制备预防和治疗肝纤维化和肝硬化的药物中的应用。研究表明，眼镜蛇毒神经生长因子可诱导HSC-T6凋亡，在细胞水平上具有抗肝纤维化作用，在动物体内也具有抗肝纤维化作用，能够有效抑制或减轻肝纤维化程度。将眼镜蛇毒神经生长因子作为药物的主要活性成分，其疗效好、起效快、安全有效、毒副作用小，是预防和治疗肝纤维化和肝硬化的理想药物。

摘要： 本发明公开了一种适于规模化生产的眼镜蛇蛇毒神经生长因子的纯化方法，是将冻干的眼镜蛇蛇毒溶解后用硫酸铵溶液进行沉淀，然后离心取上清液，采用截留分子量为3K的超滤膜膜包超滤，交换缓冲液至pH 5.0浓度为50mM的NaAc缓冲溶液，交换完缓冲液的样品上样于CM Sepharose FF柱层析，收集目的蛋白，上样于Superdex 75柱，收集目的蛋白，得到眼镜蛇蛇毒神经生长因子原液，本发明与现有技术方法相比提高了处理量和得率，适用于规模化生产。

摘要： 本发明公开了一种眼镜蛇毒因子和眼镜蛇毒神经毒素的组合分离纯化方法，是首先低温高速离心处理蛇毒原液，再使用3KDa超滤膜除去蛇毒中小分子物质和低分子多肽等，两步层析分别是CM-Sephrose FF层析柱和Superdex 200凝胶层析柱，在一次生产中分别得到眼镜蛇神经毒素和眼镜蛇毒因子两种有效成分，本发明具有可以同时分离眼镜蛇毒因子和眼镜蛇神经毒素、有效提高了眼镜蛇毒的利用效率、产品纯度高、适合工业化生产的特点。

摘要： 本发明公开了一种眼镜蛇毒因子和眼镜蛇毒神经毒素的组合分离纯化方法，是首先低温高速离心处理蛇毒原液，再使用3KDa超滤膜除去蛇毒中小分子物质和低分子多肽等，两步层析分别是CM-Sephrose FF层析柱和Superdex 200凝胶层析柱，在一次生产中分别得到眼镜蛇神经毒素和眼镜蛇毒因子两种有效成分，本发明具有可以同时分离眼镜蛇毒因子和眼镜蛇神经毒素、有效提高了眼镜蛇毒的利用效率、产品纯度高、适合工业化生产的特点。