聚山梨酯-80致RBL-2H3肥大细胞脱颗粒的研究

目的:研究聚山梨酯-80对RBL-2H3肥大细胞脱颗粒释放组胺的影响.方法:培养大鼠来源的RBL-2H3肥大细胞,取不同厂家来源的聚山梨酯-80与RBL-2H3细胞共培养60 min,用荧光分光光度法定量检测RBL-2H3细胞释放的组胺量,计算组胺释放率.结果:不同厂家来源的聚山梨酯-80与RBL-2H3细胞作用60 min后,细胞的组胺释放率与空白对照组相比均显著增加,在一定浓度范围内,组胺的释放随聚山梨酯-80浓度的增加而增加.结论:聚山梨酯-80可导致RBL-2H3肥大细胞脱颗粒,并存在着明显的量效关系,为研究聚山梨酯80致过敏反应机制提供了一定的依据.     

药用注射辅料聚山梨酯80诱发类过敏反应的细胞研究

目的:观察聚山梨酯80诱导大鼠嗜碱性粒细胞白血病细胞株RBL-2 H3细胞脱颗粒现象,探讨其诱发类过敏反应的可能机制。方法:聚山梨酯80与RBL-2 H3细胞共同孵育60 min后,透射电镜观察细胞发生脱颗粒反应的形态学变化,荧光显微镜下观察细胞膜磷脂酰丝氨酸与Annexin V结合变化,分光光度法测定细胞上清液β-氨基己糖苷酶释放百分率,并通过阿利新蓝染色试验进行定性观察。结果:不同浓度聚山梨酯80可诱导细胞发生典型的脱颗粒反应形态学变化,与阴性对照组相比脱颗粒率及组胺释放率显著升高,且具有浓度依赖性。结论:聚山梨酯80单次、首次给药即可诱导RBL-2 H3细胞脱颗粒,释放组胺,诱发类过敏反应,这可能是其临床首次用药即引起严重不良反应的机制之一。     

聚山梨酯80对多源肥大细胞脱颗粒的影响研究

目的 通过比较不同浓度聚山梨酯80溶液对RBL-2H3、P815、Ku812细胞脱颗粒的影响,探究聚山梨酯80的量与过敏反应的关系,进而筛选出一套灵敏、稳定的体外肥大细胞脱颗粒模型。方法 体外培养RBL-2H3、P815和Ku812细胞,测定3株细胞的生长曲线,在细胞生长对数期,以不同浓度（0.04、0.20、1.00、5.00、10.00、20.00、40.00、80.00 mg/mL）聚山梨酯80分别刺激3株细胞,采用中性红染色法显微镜下观察不同浓度聚山梨酯80溶液对3株细胞脱颗粒的影响,并计算脱颗粒百分率,同时以化学发光法分别检测组胺和β-氨基己糖苷酶释放率,以酶联免疫吸附法测定类胰蛋白酶的释放量;并进一步检测聚山梨酯80对人的肥大细胞IgE释放的影响。结果 3株肥大细胞脱颗粒模型中,各细胞的脱颗粒指标均随聚山梨酯80浓度的升高而升高。相同浓度聚山梨酯80对人源、大鼠、小鼠肥大细胞的类胰蛋白酶释放量无较大统计学差异;与RBL-2H3细胞系比较,P815细胞和组胺释放率显著降低（P<0.05、0.01）,Ku812细胞组胺释放率和β-氨基己糖苷酶释放率显著升高（P<0.05、0.01）,Ku812细胞脱颗粒最灵敏。但在实验过程中发现Ku812细胞模型稳定性、可重复性较差,而RBL-2H3细胞稳定性、可重复性均优于Ku812和P815细胞。0.04~80.00 mg/mL的聚山梨酯80溶液作用于Ku812细胞产生的IgE均低于检测限。结论 聚山梨酯80诱导的过敏反应可能是不经过IgE介导的类过敏反应,随着聚山梨酯80浓度的增大,3个细胞模型脱颗粒现象显著,相比于Ku812和P815细胞,RBL-2H3细胞更适合作为体外肥大细胞脱颗粒检测模型。     

参麦注射液致RBL-2H3细胞脱颗粒的研究

目的 探讨参麦注射液(SMI)对RBL-2H3细胞脱颗粒的影响及其原因。方法 以C48/80为工具药建立RBL-2H3细胞脱颗粒模型, 检测不同浓度C48/80与RBL-2H3细胞作用不同时间后细胞β-己糖苷酶、类胰蛋白酶和组胺的释放率以及细胞活力, 在细胞活力大于80%情况下, 选择释放程度较高的指标和条件为优选考察指标和条件。将SMI和其溶剂(Tween-80)原液等比稀释成不同浓度后与RBL-2H3细胞共同培养, 通过中性红染色法观察细胞脱颗粒的形态学变化, 分别用显色法和间接荧光法检测细胞上清的β-己糖苷酶和组胺释放率, 采用细胞计数法(CCK-8)检测细胞的活力。结果 RBL-2H3细胞脱颗粒模型的最佳作用时间为30 min, 最佳指标为β-己糖苷酶和组胺释放率。与空白组相比, SMI质量浓度低于13.3 g生药/L(3倍临床浓度)时, 细胞中性红染色未见脱颗粒现象, 组胺和β-己糖苷酶释放率亦无差异;而在Tween-80质量浓度为1.00 g/L时, SMI 40 g生药/L(9倍临床浓度)组和溶剂1.00 g/L组细胞中性红染色均可见脱颗粒现象, 细胞上清组胺和β-己糖苷酶释放率亦明显增加。此外, CCK-8结果显示, 与空白组相比, 各浓度的SMI对细胞活力均无影响。结论 SMI低于3倍临床浓度无明显RBL-2H3细胞脱颗粒作用;而在9倍临床浓度能刺激细胞脱颗粒, 这种脱颗粒作用可能与所含溶剂(Tween-80)有关, 与其对RBL-2H3的细胞毒性作用无关。提示SMI在低于3倍临床浓度相对安全, 在9倍临床浓度时有致类过敏反应的风险。     

紫花地丁止痒复方对RBL-2H3细胞脱颗粒的影响

目的考察紫花地丁止痒复方(Viola yedoensis makino antiitching compound,VYAC)对RBL-2H3细胞脱颗粒的影响及机制。方法CCK-8检测VYAC对RBL-2H3细胞的毒性;C48/80诱导RBL-2H3细胞发生脱颗粒,台盼蓝染色、β-氨基己糖胺酶释放、组胺释放、细胞内Ca2+浓度,评价VYAC对C48/80诱导的RBL-2H3细胞脱颗粒情况;Western blot法检测相关蛋白(Syk、p-Syk、PI3K、Akt、p-Akt)的表达。结果100 mg·L^-1的C48/80能够明显刺激RBL-2H3细胞发生脱颗粒,脱颗粒率达74%(P<0.05);VYAC呈剂量依赖性抑制β-氨基己糖胺酶和组胺的释放(P<0.05),且剂量在800 mg·L^-1以下时不影响RBL-2H3细胞存活;VYAC能够明显减弱细胞内荧光强度,降低细胞内Ca2+浓度;VYAC(25、100 mg·L^-1)明显抑制PI3K蛋白表达、抑制Syk、Akt蛋白的磷酸化(P<0.05)。结论VYAC能够抑制过敏性皮炎中肥大细胞脱颗粒,抑制Ca2+内流,其机制可能是抑制Syk/PI3K/Akt活化。     

基于RBL-2H3与P815细胞体外模型的聚山梨酯80、维生素K1注射剂、注射用两性霉素B脂质体类过敏反应潜在风险评价

目的 基于 RBL-2H3及 P815细胞系,选择 Compound 48/80（C48/80）为阳性药构建类过敏反应的体外评价模型,初步评价聚山梨酯80、维生素K₁注射剂（VK₁I）、注射用两性霉素B脂质体（ABL）导致类过敏反应的潜在风险。方法 应用 CCK-8 法检测 C48/80（10、30、60、100 μg·mL^-1）、聚山梨酯 80（2.5、5.0、10.0、50.0 mg·mL^-1）、VK₁I（0.625、1.250、2.500、5.000、10.000 mg·mL^-1）、ABL（0.125、0.250、0.500、1.000、2.000 mg·mL^-1）对 RBL-2H3、P815 细胞活性的影响,计算半数抑制浓度（IC₅₀）,阳性药及受试物均选择＜IC₅₀浓度进行后续实验;结合中性红染色形态学观察,研究阳性药及受试物的细胞毒性;流式细胞仪检测Annexin V阳性细胞率及Fluo-4AM标记率;ELISA法检测β-氨基己糖苷酶（β-Hex）及组胺释放量。结果 中性红染色结果显示,在C48/80作用下RBL-2H3、P815细胞部分皱缩或者偶有破损,但大部分细胞仍维持完整细胞形态;在聚山梨酯 80、ABL、VK₁I高浓度的作用下,RBL-2H3、P815细胞大部分仍能保持正常形态。C48/80在＜IC₅₀浓度时能够引起较强的细胞脱颗粒反应,模型建立成功。聚山梨酯80、VK₁I在＜IC₅₀浓度时均出现了浓度相关性细胞脱颗粒现象,与对照组比较,2种细胞聚山梨酯80 2.5、5.0 mg·mL^-1组及VK₁I 0.75、1.50、3.00 mg·mL^-1组Annexin V阳性率、Fluo-4AM标记率均显著升高（P＜0.05、0.01）;聚山梨酯 80 2.5、5.0 mg · mL^-1 组及 VK₁I 1.5、3.0 mg·mL^-1组的组胺、β-Hex释放量显著升高（P＜0.05、0.01）。ABL 组 Annexin V 阳性率浓度相关性升高趋势不明显 ,与对照组比较 ,仅 P815 细胞 ABL 2.00 mg·mL^-1组显著升高（P＜0.05）,且升高幅度不大 ;与对照组比较 ,2种细胞ABL 1、2 mg·mL^-1组的Fluo-4AM标记率和组胺、β-Hex释放量显著升高（P＜0.05、0.01）。结论 聚山梨酯80、VK₁I高浓度具有导致类过敏反应产生风险,ABL 还需进一步研究。     

RBL-2H3细胞不适合用于类过敏模型的建立

目的考察RBL-2H3细胞是否适用于建立类过敏反应模型。方法用荧光定量聚合酶链反应考察RBL-2H3细胞上Mas相关G蛋白偶联受体(Mas-related G protein cou-pled receptor,Mrgpr)B2的表达情况;用显微镜观察和MTS法考察Compound 48/80对RBL-2H3细胞活力的影响;测定不同浓度Compound 48/80刺激RBL-2H3细胞脱颗粒释放的β-己糖胺酶含量,对比RBL-2H3细胞、人肥大细胞系LAD2和大鼠腹腔肥大细胞(rat peritoneal mast cells,RPMCs)对Compound 48/80响应性的差异。结果RBL-2H3细胞可表达MrgprB2受体。Compound 48/80能剂量依赖性地诱导RBL-2H3细胞释放β-己糖胺酶,但在高剂量(≥20 mg·L^-1)时对RBL-2H3的细胞活力产生明显影响,此时释放的β-己糖胺酶应当是由于其细胞毒作用引起细胞破裂所致。同在无毒剂量(10 mg·L^-1)的Compound 48/80刺激下,LAD2和RPMCs的响应性良好,β-己糖胺酶释放量分别为空白对照的15.02倍和16.05倍,而RBL-2H3细胞仅为空白对照的2.35倍。结论RBL-2H3细胞对Compound 48/80的响应性差,表明其并不适用于建立类过敏反应模型。     

非免疫性过敏反应细胞模型的建立

目的:通过非免疫性刺激物C48/80诱导大鼠嗜碱性粒细胞白血病细胞株RBL-2H3细胞脱颗粒反应正交试验,优化非免疫性过敏反应细胞模型建立条件.方法:在不同的孵育时间下,C48/80与不同浓度的RBL-2H3细胞共孵育,通过测定β-氨基己糖苷酶的释放率确定建立非免疫型过敏反应细胞模型的最优实验条件,并且分析不同检测方法间的差异.结果:不同浓度、不同孵育时间下的RBL-2H3细胞均可受C48/80诱导发生典型的脱颗粒反应,但不同条件下的脱颗粒程度和β-氨基己糖苷酶释放率都有显著差异.结论:当RBL-2H3细胞浓度为2×105 mL、孵育时间60 min时,细胞的感受性较好,其脱颗粒程度与药物浓度呈正相关.     

毛冬青注射液细胞毒性及类过敏反应的评价

目的:研究毛冬青注射液的安全性,为临床合理用药提供参考.方法;通过L-929细胞毒性实验和RBL-2H3细胞脱颗粒实验,考察毛冬青注射液的临床毒性大小以及是否存在类过敏的不良反应.结果:毛冬青注射液在高浓度时(333 μl·ml-1)抑制细胞增殖,低浓度时(111 μl· ml-1)促进细胞增殖,并有浓度依赖性,同时会引起部分RBL-2H3细胞脱颗粒.结论:细胞毒性实验可用于评价药物的毒性大小;细胞脱颗粒实验可用于评价药物的类过敏反应.     

牛膝多糖对抗原诱导的肥大细胞活化的影响

目的观察牛膝多糖(achyranthes bidentata polysaccha-rides,ABPS)对肥大细胞活化脱颗粒的影响。方法运用大鼠被动皮肤过敏反应(PCA)实验,用比色测定法检测ABPS在体内对肥大细胞(MC)影响;体外实验将ABPS分为高、中、低3个剂量组,然后分别将其加入抗原致敏的RBL-2H3细胞中(大鼠嗜碱性粒细胞白血病细胞,国际公认的MC研究模型细胞),观察ABPS对RBL-2H3细胞脱颗粒的影响。结果ABPS能明显抑制大鼠PCA、RBL-2H3细胞脱颗粒,并能抑制RBL-2H3细胞释放组胺、肿瘤坏死因子α及白细胞介素4;抑制RBL-2H3细胞中Akt和p38的磷酸化。结论ABPS的抗过敏作用与抑制肥大细胞的脱颗粒及炎性物质释放有关;ABPS抑制肥大细胞的活化与抑制Akt和p38的活性相关。     

中药注射剂所含吐温-80与过敏反应关系的研究

目的：观察不同浓度吐温-80溶液、吐温-80含量不同的中药注射剂对RBL-2H3细胞脱颗粒的影响,探讨中药注射剂所含吐温-80与过敏反应的关系。方法：体外培养RBL-2H3细胞,加入不同浓度（40、20、10、2、1、0.2、0.1、0.05mg/mL）的吐温-80溶液,之后加中性红染液,计数不同浓度吐温-80溶液各组及对照组的脱颗粒细胞,并计算其百分率,同时检测细胞上清液中β-氨基己糖苷酶及组胺的释放量;测定穿琥宁注射液和香丹注射液中吐温-80的含量,2种中药注射剂对RBL-2H3细胞的半数抑制浓度（IC50）以及加入2种注射液各组细胞释放组胺的量。结果：中性红染色实验显示吐温-80可导致RBL-2H3细胞脱颗粒,表现为肥大细胞体积变大,内有空泡产生;浓度为40、20、10、2、1、0.2、0.1mg/mL的吐温-80溶液各组和RPMI1640对照组导致细胞的脱颗粒百分率分别为（57.38±0.47）、（32.54±2.33）、（21.74±0.72）、（16.96±0.26）、（11.40±1.70）、（9.71±0.26）、（7.22±0.15）和（1.51±1.39）%,2组相比差异有统计学意义（P〈0.05,P〈0.01）;浓度为40、20、2、1、0.2mg/mL的吐温-80溶液各组和RPMI1640对照组致细胞β-氨基己糖苷酶的释放率分别为（52.44±1.53）、（18.91±0.77）、（7.50±1.82）、（6.65±0.20）、（6.15±0.27）和（0.35±0.06）%,2组相比差异有统计学意义（P〈0.05,P〈0.01）;不同浓度吐温-80溶液引起RBL-2H3细胞释放组胺的量也不同;当吐温-80溶液浓度为20～0.1mg/mL时,RBL-2H3细胞脱颗粒百分率、β-氨基己糖苷酶的释放率及其释放组胺的量均与吐温-80溶液的浓度呈线性关系（r=0.9862,r=0.9849,r=0.9740）。穿琥宁注射液和香丹注射液中吐温-80的含量分别为（0.086±0.004）和（0.070±0.008）mg/mL,2种注射液对RBL-2H3细胞的IC50分别为（57.4±1.2）、（1.0±0.2）μL/mL,穿琥宁注射液和香丹注射液组组胺释放量分别为（2.39±0.01）和（1.87±0.00）ng/mL。结论：吐温-80可引起RBL-2H3细胞脱颗粒释放炎症介质;RBL-2H3细胞组胺的释放量与中药注射剂中吐温-80的含量有关;中药注射剂中所含的吐温-80可能与过敏反应的发生有关。     

中药制剂苓槐丸提取物对小鼠过敏性皮炎的治疗作用及机制研究

目的研究中药制剂苓槐丸对过敏性皮炎的治疗作用及机制。方法制备苓槐丸甲醇提取物（MELH）,观察其对过敏性皮炎模型鼠耳肿胀程度及炎症因子释放的影响;而后,检测MELH 对肥大细胞RBL鄄2H3 脱粒作用及细胞信号通路的影响。结果MELH 可有效抑制过敏性皮炎模型鼠耳炎症性肿大（P 〈0. 05）,及抑制鼠耳组织中IFN-γ和TNF-α水平升高（P 〈0. 05）。MELH 可剂量依赖性抑制佛波酯（PMA）和钙离子载体（A23187）联合引起的RBL鄄2H3 细胞的组胺释放（P〈0. 05）和p38 MAPK 磷酸化。结论MELH 通过抑制T 细胞炎症因子的释放、肥大细胞脱粒作用及p38 MAPK 通路的活化,阻止T细胞向Th1免疫偏离,总体说苓槐丸可起到明显的抗过敏性皮炎作用。     

Mast cell degranulation induced by chlorogenic acid

Aim:

To investigate the mechanism of chlorogenic acid (CA)-induced anaphylactoid reactions.

Methods:

Degranulation of peritoneal mast cells was assayed by using alcian blue staining in guinea pigs, and the degranulation index (DI) was calculated. CA-induced degranulation of RBL-2H3 cells was also observed and assayed using light microscopy, transmission electron microscopy, flow cytometry, and β-hexosaminidase release.

Results:

CA 0.2, 1.0, and 5.0 mmol/L was able to promote degranulation of peritoneal mast cells in guinea pigs in vitro, but it did not increase the degranulation of peritoneal mast cells in CA-sensitized guinea pigs compared with control (P>0.05). Treatment with CA 0.2, 1.0, and 5.0 mmol/L for 30, 60, and 120 min induced degranulation in RBL-2H3 cells in a dose- and time-dependent manner (P<0.01). Under transmission electron microscope typical characteristics of degranulation, including migration of granular vesicles toward the plasma membrane and integration combined with exocytosis, were observed, after CA or C48/80 treatment. Fluorescent microscopy and flow cytometric analysis showed that CA induced concentration-dependent translocation of phosphatidylserine in RBL-2H3 cells. β-hexosaminidase release in RBL-2H3 cells was significantly increased after incubation with 1 mmol/L CA for 60 min and 5 mmol/L CA for 30 min (P<0.01).

Conclusion:

CA induces degranulation of peritoneal mast cells and RBL-2H3 cells in guinea pigs, which might be one of the mechanisms of the generation of anaphylactoid reactions induced by CA.     

G protein coupled receptor specificity for C3a and compound 48/80-induced degranulation in human mast cells: roles of Mas-related genes MrgX1 and MrgX2

Although human mast cells express G protein coupled receptors for the anaphylatoxin C3a, previous studies indicated that C3a causes mast cell degranulation, at least in part, via a C3a receptor-independent mechanism similar to that proposed for polycationic molecules such as compound 48/80. The purpose of the present study was to delineate the receptor specificity of C3a-induced degranulation in human mast cells. We found that C3a, a C3a receptor "superagonist" (E7) and compound 48/80 induced Ca(2+) mobilization and degranulation in a differentiated human mast cell line, LAD2. However, C3a and E7 caused Ca(2+) mobilization in an immature mast cell line, HMC-1 but compound 48/80 did not. We have previously shown that LAD2 cells express MrgX1 and MrgX2 but HMC-1 cells do not. To delineate the receptor specificity for C3a and compound 48/80 further, we generated stable transfectants expressing MrgX1 and MrgX2 in a rodent mast cell line, RBL-2H3 cells. We found that compound 48/80 caused degranulation in RBL-2H3 cells expressing MrgX1 and MrgX2 but C3a did not. By contrast, E7 activated RBL-2H3 cells expressing MrgX2 but not MrgX1. These findings demonstrate that in contrast to previous reports, C3a and compound 48/80 do not use a shared mechanism for mast cell degranulation. It shows that while compound 48/80 utilizes MrgX1 and MrgX2 for mast cell degranulation C3a does not. It further reveals the novel finding that the previously characterized synthetic peptide, C3a receptor "superagonist" E7 activates human mast cells via two mechanisms; one involving the C3a receptor and the other MrgX2.     

Ephedrae herba (Mao) decreased histamine content in RBL-2H3 cells

The effect of Ephedrae herba (Mao) on histamine content was investigated. When rat basophilic leukemia (RBL-2H3) cells were incubated for 48 h with Mao, Mao decreased histamine content in a concentration-dependent manner. However, the ratio of released histamine to total histamine was scarcely affected by Mao treatment when RBL-2H3 cells were stimulated by ionomycin. On the other hand, the content of -hexosaminidase, another marker of degranulation, was only slightly decreased by Mao. The expression level of the active form (53 kDa) of l-histidine decarboxylase, the enzyme which synthesizes histamine, was partially suppressed by Mao. Furthermore, Mao significantly suppressed proliferation of RBL-2H3 cells in a concentration-dependent manner. The phosphodiesterase inhibitor 3-isobutyl-1-methylxanthine revealed an increasing effect of Mao on cAMP level in RBL-2H3 cells. Since this result suggested that Mao may stimulate adenylate cyclase, we evaluated the effect of adenylate cyclase inhibitor SQ 22536 on Mao-induced decrease in histamine content. As a result, we showed that SQ 22536 did not have a reducing effect of Mao. From these results it is understood that Mao decreased histamine content by inhibiting cell proliferation and expression of histidine decarboxylase. However, these effects are not related to the increase in cAMP.     

In vitro and in vivo antiallergic effect of the fructus of Evodia rutaecarpa and its constituents

The unripe fruit of Evodia rutaecarpa (JUSS) BENTH (ER, Family Rutaceae) has been used frequently as a traditional medicine against inflammatory diseases in Korea, China and Japan. To evaluate antiallergic effect of ER, we isolated its main constituents, evodiamine and rutaecarpine, and evaluated in vivo their inhibitory effects against passive cutaneous anaphylaxis (PCA) reaction induced by IgE-antigen complex and scratching behaviors by compound 48/80. ER and its constituents, evodiamine and rutaecarpine, potently inhibited PCA reaction and scratching behaviors in mice, although ER weakly inhibited scratching behaviors. Evodiamine and rutaecarpine inhibited TNF-alpha and IL-4 protein expression in RBL-2H3 cells induced by IgE-antigen complex, although these did not inhibit degranulation of RBL-2H3 cells induced by IgE-antigen complex and rat peritoneal mast cells induced by compound 48/80. These findings suggest that ER and its constituents, evodiamine and rutaecarpine, may be effective for IgE-induced allergic diseases such as atopic dermatitis and rhinitis.     

The relation between degranulation and rapid metabolic responses in RBL-2H3 cells

The relation between degranulation and rapid metabolic responses (acidification rate changes) in RBL-2H3 cells was studied using a cytosensor microphysiometer, a silicon-based biosensor system. The metabolic responses in RBL-2H3 cells by antigen stimulation were compared with those by inhibitors of Ca2+ -ATPase. The former resulted in a rapid transient increase in the acidification rate of RBL-2H3 cells while the latter resulted in gradual decreases. When RBL-2H3 cells were costimulated with the inhibitors of Ca2+ -ATPase and an activator (PMA, phorbol-12-myristoyl-13-acetate) of protein kinase C, the metabolic responses increased again in RBL-2H3 cells. This seems to indicate that degranulation in RBL-2H3 cells was accelerated by costimulation with the inhibitors and PMA. However, costimulation was not able to completely mimic the way antigen stimulated RBL-2H3 cells in degranulation and in rapid metabolic responses.