Effect of recombinant human interleukin-11 on expressions of interleukin-11 receptorα-chain and glycoprotein 130 in intestinal epithelium cell line-6 after neutron irradiation

AIM： To explore the effect of recombinant human interleukin-11 （rhIL-11） on the expressions of interleukin-11 receptor α-chain （IL-11Rα） and an additional signal transducer glycoprotein 130 （gp130） in intestinal epithelium cell line-6 （IEC-6） after neutron irradiation. METHODS： Cultured IEC-6 cells were exposed to 4.0Gy neutron and treated with 100 ng/mL rhIL-11 12 h prior to or immediately after irradiation. The apoptosis and necrosis rates and expressions of IL-11Rα and gp130 were observed by flow cytometry, immunohistochemistry, Western blot and image analysis. RESULTS： The apoptosis rate of IEC-6 cells was increased by irradiation at 6 h （P 〈 0.01）, IL-11 stimulation resulted in a decreased apoptosis rate in irradiated IEC-6 cells （P 〈 0.05）. In normal control IEC-6 cells, intense immunoreactivity of IL-11Rα was located within the cell membrane and cytoplasm. The level of IL-11Rα expression significantly decreased at 6 h after irradiation （P 〈 0.01） and restored at 24 h after irradiation. In IEC-6 cells treated with both radiation and rhIL-11, the level of IL- 11Rα expression was higher than that of irradiated cells （P 〈 0.05）. When it came to gp130 protein, it was located in the cytoplasm of IEC-6 cells. After irradiation, we found a progressive decrease in the expression of gp130 protein （P 〈 0.05） in 48 hours post-radiation, while in rhIL-11-stimulated cells, it came back to normal level at 24 h after irradiation and decreased at 48 h, but was still higher than that of only irradiated cells （P 〈 0.05）. CONCLUSION： rhIL-11 can protect IEC-6 cells from neutron irradiation. The protective effect of rhIL-11 might be connected with its ability to up-regulate the expressions of specific ligand-binding subunit IL-11Rα and signal-transducing subunit gp130.

Interleukin-13 inhibits cytokines synthesis by blocking nuclear factor-κB and c-Jun N-terminal kinase in human mesangial cells

Objective： Monocytes/macrophages, proinflammatory cytokines and chemokines are important in the pathogenesis of glomerulonephritis. Interleukin （IL） -13 has been shown to exert potent anti-inflammatory properties. This study was designed to investigate the effect of IL-13 on the expression of proinflammatory cytokines, chemokines and profibrogenic cytokines and the involved molecular mechanism in cultured human mesangial cells （HMCs）. Methods： The expressions of proinflammatory cytokines, chemokines and profibrogenic cytokines were determined by ribonuclease protection assay （RPA）. Activity of nuclear factor-kappa B （NF-κB） and activa- tor protein-1 （AP-1） was examined by electrophoretic mobility shift assay （EMSA）. NF-κB subunit p65 nuclear transportation and c-Jun N-terminal kinase （JNK） activity were assayed by immunoblot. Results： Recombinant IL-13 inhibited tumor necrosis factor-α （TNF-u）, IL-1α, IL-1β, monocyte chemoattractant protein-1 （MCP-1）, IL-8, and transforming growth factor-β1 （TGF-β1） mRNA expressions in a dose-dependent manner. Lipopoly- sacchorides （LPS） dramatically increased NF-κB DNA binding activity of HMCs, which was inhibited by IL-13 in a dose-dependent manner. LPS-activated NF-κB contained p50 and p65 dimers, but not c-Rel subunit. IL-13 blocked LPS-induced NF-κB subunit p65. LPS stimulated JNK/AP-1 activation, which was inhibited by IL-13 in a dose-dependent manner. Conclusion： IL-13 inhibits proinflammatory cytokines, chemokines, and profibrogenic cytokines synthesis by blocking NF-κB and JNK/AP-1 activation. These observations point to the importance of IL-13 in the modulation of inflammatory processes in the renal glomerulus.

Interleukin-13 promotes cellular senescence through inducing mitochondrial dysfunction in IgG4-related sialadenitis

Immunoglobulin G4-related sialadenitis(IgG4-RS)is an immune-mediated fibro-inflammatory disease and the pathogenesis is still not fully understood.The aim of this study was to explore the role and mechanism of interleukin-13(IL-13)in the cellular senescence during the progress of IgG4-RS.We found that the expression of IL-13 and IL-13 receptorα1(IL-13Rα1)as well as the number of senescent cells were significantly higher in the submandibular glands(SMGs)of IgG4-RS patients.IL-13 directly induced senescence as shown by the elevated activity of senescence-associatedβ-galactosidase(SA-β-gal),the decreased cell proliferation,and the upregulation of senescence markers(p53 and p16)and senescence-associated secretory phenotype(SASP)factors(IL-1βand IL-6)in SMG-C6 cells.Mechanistically,IL-13 increased the level of phosphorylated signal transducer and activator of transcription 6(p-STAT6)and mitochondrial-reactive oxygen species(mt ROS),while decreased the mitochondrial membrane potential,ATP level,and the expression and activity of superoxide dismutase 2(SOD2).Notably,the IL-13-induced cellular senescence and mitochondrial dysfunction could be inhibited by pretreatment with either STAT6 inhibitor AS1517499 or mitochondria-targeted ROS scavenger Mito TEMPO.Moreover,IL-13 increased the interaction between p-STAT6 and c AMP-response element binding protein(CREB)-binding protein(CBP)and decreased the transcriptional activity of CREB on SOD2.Taken together,our findings revealed a critical role of IL-13 in the induction of salivary gland epithelial cell senescence through the elevated mitochondrial oxidative stress in a STAT6–CREB–SOD2-dependent pathway in IgG4-RS.

Apelin-13通过NLRP3/caspase-1/GSDMD通路抑制脑缺血再灌注损伤小鼠细胞焦亡

目的:探究Apelin-13调节肽对脑缺血再灌注(I/R)损伤模型小鼠神经细胞焦亡的影响。方法:利用大脑中动脉栓塞再灌注法(MCAO/R)制备小鼠I/R损伤模型,氧糖剥夺/复氧(OGD/R)法制备HT22细胞损伤模型,同时给予Apelin-13处理。神经功能缺损评分评估小鼠神经功能;苏木精-伊红染色法(HE)和尼氏染色观察小鼠脑梗死区组织形态变化;2,3,5氯化三苯基四氮唑(TTC)染色观察脑梗死体积;Western Blot检测梗死区脑组织或者HT22细胞中NOD样受体热蛋白结构域相关蛋白3(NLRP3)、消皮素D(GSDMD)、胱天蛋白酶1(caspase-1)、凋亡相关斑点样蛋白(ASC)、白细胞介素1β(IL-1β)和白细胞介素18(IL-18)等分子的表达;酶联免疫吸附实验(ELISA)检测小鼠血清及培养上清中IL-1β和IL-18的水平;用CCK-8试剂盒和乳酸脱氢酶(LDH)检测试剂盒分别检测HT22细胞活性和细胞损伤;caspase-1活性检测试剂盒检测HT22细胞中caspase-1的活性;免疫荧光染色观察HT22细胞中caspase-1和GSDMD表达。结果:Apelin-13可显著改善I/R小鼠神经功能和脑梗死体积,减轻梗死区病理损伤。同时降低血清中IL-1β和IL-18的水平。此外,Apelin-13可降低小鼠脑梗死区NLRP3、GSDMD、caspase-1、IL-1β、IL-18等分子的表达。体外实验表明Apelin-13可显著增加OGD/R处理的HT22细胞活力,降低caspase-1活性,并减少LDH含量,同时降低OGD/R处理的HT22细胞中NLRP3、GSDMD、caspase-1、IL-1β、IL-18等分子的表达。结论:Apelin-13可通过NLRP3/caspase-1/GSDMD通路抑制脑缺血再灌注损伤小鼠细胞焦亡,进而发挥神经保护作用。

6-Gingerol, asarinin, and deoxyschizandrin improve bronchial epithelium functions in an interleukin-13einduced BEAS-2B cell model

Objective:To explore the effects of 6-gingerol,asarinin,and deoxyschizandrindthe main components of Zingiber officinale(Willd.)Rosc.(Gan Jiang),Asarum heterotropoides f.var.mandshuricum(Maxim.)(Xi Xin),and Schisandra chinensis(Turcz.)Baill.(Wu Wei Zi),respectivelydon an interleukin(IL)-13einduced BEAS-2B cell model in vitro.Methods:The BEAS-2B cell model was established using 25 ng/mL IL-13 combined with 1%fetal bovine serum(FBS)in vitro.Mitoquinone mesylate(Mito-Q)treatment was used as a positive control group,and different concentrations of 6-gingerol,asarinin,and deoxyschizandrin were used to treat the models.The level of reactive oxygen species(ROS)production was detected by flow cytometry.The expression levels of LC3B,Beclin1,adenosine 50-monophosphate(AMP)eactivated protein kinase(AMPK),phosphory-lated-AMPeactivated protein kinase(P-AMPK),dynamin-related protein 1(DRP1),and mitochondrial fusion protein 2(MFN2)were detected by Western blot.Mitochondrial membrane potential(MMP)assay kit with JC-1 was utilized to detect the level of MMP.Results:The BEAS-2B cells exposed to 25 ng/mL IL-13 with 1%FBS showed an increased ROS level and a decreased MMP.6-Gingerol,asarinin,and deoxyschizandrin were able to downregulate ROS level and upregulate the MMP in the BEAS-2B model.Asarinin and deoxyschizandrin reduced the expression of autophagy protein LC3B,while deoxyschizandrin significantly increased the expression of DRP1 in the BEAS-2B model.Conclusion:6-Gingerol,asarinin,and deoxyschizandrin can reduce ROS generation and increase MMP,but have different regulatory effects on the expression of autophagy protein and mitochondrial mitotic protein.The three components have both synergistic and complementary effects in classic medicine compatibility.This study may provide an innovative strategy to reduce the lung inflammation related to IL-13.

Interleukin-13 and age-related macular degeneration

AIM：To identify the effects of interleukin（IL）-13 on retinal pigment epithelial（RPE） cells and the IL-13 level in aqueous humor of age-related macular degeneration（AMD） patients.METHODS：IL-13 levels in aqueous humor specimens from AMD patients were detected with enzyme-linked immunosorbent assay（ELISA）.ARPE-19 cells were treated with 10 ng/m L IL-13 for 12,24,and 48 h.The cell proliferaton was evaluated by the MTS method.The m RNA and protein levels of α-SMA and ZO-1 were evaluated with quantitative real-time polymerase chain reaction（q RT-PCR） and Western blot respectively.The expression of tumor necrosis factor-α（TNF-α）,transforming growth factor-β（TGF-β） and vascular endothelial growth factor（VEGF） were assessed by ELISA.RESU LTS：IL-13 levels in the aqueous humor of patients with AMD were significantly higher than those in the control（167.33±17.64 vs 27.12±5.65 pg/m L;P〈0.01）.In vit ro,IL-13 of high concentrations（10,15,and 20 ng/m L） inhibited ARPE-19 cell proliferation.α-SMA m RNA in ARPE-19 cell were increased（1.017±0.112 vs 1.476±0.168;P〈0.001） and ZO-1 decreased（1.051±0.136 vs 0.702±0.069;P〈0.001） after treated with 10 ng/m L IL-13 for 48 h.The protein expression of α-SMA and ZO-1 also showed the same tendency（α-SMA：P=0.038;ZO-1：P=0.008）.IL-13 significantly reduced the level of TNF-α（44.70±1.67 vs 31.79±3.53 pg/m L;P=0.005） at 48 h,but the le vel of TGF-β2 was significantly increased from 34.44±2.92 to 57.61±6.31 pg/m L at 24h（P=0.004） and from 61.26±1.11 to 86.91±3.59 pg/m L at 48h（P〈0.001）.While expressions of VEGF didn＇t change after IL-13 treatment.CONCLUSION：IL-13 in vitr o inhibit ARPE-19 cell proliferation and expression in the aqueous may be associated with AMD.

Determination of Serum Interleukin-13 and Nerve Growth Factor in Patients with Systemic Lupus Erythematosus and Clinical Significance

The changes in the levels of serum interleukin-13 (IL-13) and nerve growth factor (NGF) in patients with systemic lupus erythematosus (SLE) and their clinical significance were investigated. Sandwich ELISA was used to determine the levels of serum IL-13 and NGF in 35 SLE patients and 15 normal controls. The results showed that the levels of serum IL-13 (92.69±9.87 pg/ml) and NGF (339.69±25.60 pg/ml) in active SLE patients were significantly higher than those in inactive SLE patients (IL-13, 54.22±9.31 pg/ml; NGF, 300.89±33.51 pg/ml)(P<0.01). The inactive patients also had significantly increased serum levels of IL-13 and NGF as compared with normal controls (IL-13, 35.20±12.70 pg/ml; NGF, 111.40±32.54 pg/ml; P<0.05 and P<0.01, respectively). Spearman correlation analysis revealed that the serum IL-13 levels were correlated with disease activity index of SLE (SLEDAI), ESR and serum levels of C_3 (r= 0.813, 0.504, -0.605, respectively). The serum NGF levels were also correlated with above markers (r=0.442, 0.338, -0.463, respectively). The serum levels of IL-13 and NGF had a positive correlation (r=0.506, P<0.01). It was suggested that IL-13 and NGF might be involved in the pathogenesis of SLE and closely correlated with disease activity.

中高温热泵混合工质R13I1/R290/R600a替代R134a的理论研究

针对普通R134a热泵制取中高温热水过程中存在的冷凝压力过高、系统效率低、不环保及无法直接替代等问题，提出一种新型中高温热泵混合工质R13I1／R290／R600a。建立基于该工质的热力循环模型，计算该循环的热力特性。结合气象数据，对其进行多工况计算并与已有的工质R134a、MIX1和MIX2对比分析。研究结果表明该新型混合工质的循环性能与同模型常温热泵工况下R134a的循环性质大致相同，且其环境性能优良：ODP为零，GWP小于20，温度滑移小于4℃。单位容积制热量略低于R134a，分别比MIX1和MIX2平均高16．7％、1．3％；COP分别比R134a、MIXI和MIX2平均高9．2％、4．1％和0．7％。综合循环性能较对比工质更优越，适用于冷凝温度为70～90℃，循环温升低于75℃的热泵工况。

新型混合制冷剂R1270/R152a/R13I1的理论研究

针对制冷剂R22的替代问题,提出了一种适用于空调等制冷设备的环保型混合制冷剂R1270/R152a/R13I1。基于Refprop8.0,对R1270/R152a/R13I1的基本热物理性质和制冷系统循环性能进行了分析,研究表明:在标准工况下,R1270/R152a/R13I1混合制冷剂的COP和单位容积制冷量均与R22相当,非常有利于直接灌注式替代;在变工况下,R1270/R152a/R13I1的滑移温度较小,性能优于R407C,单位容积制冷量与R407C和R22相当,是一种优良的R22替代物。

小鼠sIL-13Rα2在毕赤酵母菌中的表达及初步活性分析

目的:克隆并在毕赤酵母中表达小鼠sIL-13Rα2基因。方法:从小鼠脾脏细胞中提取总RNA,逆转录为cDNA,应用分段PCR的方法将sIL-13Rα2基因定向克隆至酵母表达质粒pPICZα-A,并转染至毕赤酵母菌表达系统进行目的蛋白表达。目的蛋白行SDS-PAGE和Western分析。结果:克隆出可溶性IL-13Rα2目的基因片段,构建重组pPICZα-A/sIL-13 Rα2表达载体,成功转染至毕氏酵母菌,诱导表达出可溶性IL-13Rα2目的蛋白。结论:已成功克隆并在毕赤酵母中表达了小鼠可溶性IL-13Rα2目的基因,为应用sIL-13Rα2蛋白治疗哮喘及其他过敏性疾病奠定了基础。

哮喘患儿血清中sIL-2R、IL-2、IL-4、IL-13的水平变化与临床意义

目的探讨哮喘患儿血清中可溶性白细胞介素-2受体(sIL-2R)、白细胞介素-2(IL-2)、白细胞介素-4(IL-4)、白细胞介素-13(IL-13)的水平变化及其与哮喘发病机制的关系。方法每例样本均取空腹静脉血并即时分离血清1ml,用ELISA法检测血清中sIL-2R、IL-2、IL-4、IL-13的水平并对结果进行统计学分析。结果哮喘急性发作组、缓解组的血清中sIL-2R、IL-2、IL-4、IL-13的结果与正常对照组比较差异均有显著性(P<0.05)。其中哮喘急性发作组、缓解组血清中sIL-2R、IL-4、IL-13的结果要明显高于正常对照组,而IL-2则明显低于正常对照组。此外,哮喘急性发作组与缓解组血清中IL-2、IL-4、IL-13的结果相比较差异均有显著性(P均<0.05),而SIL-2R则无明显差异。结论哮喘患儿血清中sIL-2R、IL-2、IL-4、IL-13的水平伴随病情进展发生显著的变化,说明它们在哮喘的免疫病理过程中起着重要的作用。

IRIS ^(13)C-美沙西汀呼气试验和ICG试验对肝硬化肝功能评估比较

目的:比较13C-美沙西汀呼气试验与吲哚氰绿(ICG)试验评估肝硬化患者肝功能状况的临床价值. 方法:肝硬化患者59例,隔夜空腹进行13C-美沙西汀呼气试验,通过红外线同位素能谱分析仪(IRIS)检测服药前、后120 min内各个时间点呼气中13CO2的含量, 得出mvmax40(40 min前的13CO2代谢速率峰值),cum40 (40 min的13CO2累积呼出丰度)和cum120(120 min的13CO2累积呼出丰度),同时进行ICG试验测定15 min 的血清ICG滞留率(R15ICG). 结果:13C-关沙西汀呼气试验的mvmax40,cum40和cum120 值在肝硬化各组之间差异具有显著性(mvmax40A-B, B—C和A-C间t值分别为2.80,4.82和10.38;cum40各组间t值分别为3.85,3.39和8.64;cum120各组间t值分别为4.52,3.75和12.36,P<0.01);R15 ICG测定值在肝硬化A,B与A,C组间差异具有显著性(t值分别为- 4.72和-1.27,P<0.01),B,C组间差异无显著性(t 值为-5.85,P>0.05).13C-美沙西汀呼气试验的mvmax40,cum40和cum120值和R15ICG测定值与Child—Pugh 肝功能分级评分均呈显著相关(r值分别为-0.562,- 0.614,-0.71 6和0.555,P<0.001).13C-美沙西汀呼气试验与Child—Pugh肝功能分级在判定肝硬化患者肝功能状况上的一致性(Kappa=0.69,P<0.05)优于ICG 试验(Kappa=0.47,P<0.05). 结论:ICG试验为评估肝硬化肝功能状况的较好定量检测方法;13C-美沙西汀呼气试验是反映肝细胞损害情况和储备功能的良好肝功能试验,对肝硬化尤其失代偿患者较之ICG试验更为灵敏.

IL-13对A549细胞IL-13Rα2表达及增殖和迁移的影响

目的探讨IL-13对人肺腺癌细胞(A549)IL-13受体α2(IL-13Rα2)表达及增殖、迁移的影响。方法采用定量逆转录聚合酶链式反应(qRT-PCR)、Western blot法检测IL-13刺激A549细胞后,检测IL-13Rα2的转录和蛋白质表达水平;酶联免疫吸附实验(ELISA)检测细胞培养上清液中的可溶型IL-13受体α2(sIL-13Rα2)含量;流式细胞术(FCM)检测胞膜型IL-13受体α2(memIL-13Rα2)、胞内型IL-13受体Rα2(iIL-13Rα2)的细胞数。MTT法、Transwell实验和细胞划痕实验观察IL-13对A549细胞增殖及迁移作用的影响。结果 A549细胞可表达IL-13Rα2,并且IL-13在较低质量浓度(10、20 ng·mL^(-1))时能上调A549细胞IL-13Rα2的表达水平,而对增殖和迁移无显著影响;在较高质量浓度(50、100 ng·mL^(-1))时对IL-13Rα2的上调作用不明显,但能促进细胞增殖和迁移。另外低质量浓度IL-13(10、20 ng·mL^(-1))对IL-13Rα2整体水平、sIL-13Rα2、memIL-13Rα2以及iIL-13Rα2的表达均有不同程度的上调(P<0.05);高质量浓度IL-13(50、100 ng·mL^(-1))刺激条件下IL-13Rα2整体水平的上调不明显且不再有剂量依赖性,sIL-13Rα2水平无明显改变、memIL-13Rα2表达略有增加、iIL-13Rα2水平明显下调(P<0.05)。结论IL-13对人肺腺癌A549细胞IL-13Rα2表达水平及增殖、迁移的影响具有双相性和差异性;IL-13Rα2在肺腺癌A549中发挥抑制IL-13促细胞增殖和迁移的作用。

sIL-13Rα2抑制IL-13介导的NIH-3T3胶原I的合成及血吸虫病肝组织中sIL-13Rα2/IL-13的表达(英文)

目的研究在成纤维细胞NIH-3T3中IL-13可溶性受体sIL-13Rα2对IL-13的抑制作用,为进一步研究sIL-13Rα2对日本血吸虫感染小鼠体内肝纤维化的治疗作用奠定基础。方法用ELISA和RT-PCR检测感染日本血吸虫的BALB/c小鼠0、6、8、10和12w不同感染时期肝脏组织IL-13和sIL-13Rα2表达和转录水平。构建sIL-13Rα2表达质粒转染成纤维细胞NIH-3T3,用IL-13(50ng/mL)刺激转染后成纤维细胞NIH-3T3,用RT-PCR和Western blotting分别检测该细胞分泌的Ⅰ型胶原。结果感染后小鼠肝脏肉芽肿组织中IL-13和sIL-13Rα2的蛋白表达水平随感染时间的延长而逐渐增高,第8wIL-13水平达到高峰(16.1586pg/mL),随后逐渐降低但仍高于正常水平(3.4146pg/mLP=0.017);第10wsIL-13Rα2的分泌达到高峰(4827.426pg/mL),以后逐渐减低,但仍高于正常水平(4057.112pg/mLP=0.021)。IL-13和sIL-13Rα2的mRNA转录趋势和ELISA检测结果相符合,均随感染时间的延长而增高,分别在第8w和第10w达到最高峰,随后逐渐降低但仍高于正常组小鼠(P=0.033;P=0.025)。实验组(sIL-13Rα2=2mg/mL)Ⅰ型胶原mRNA转录水平较正常对照组减低8.83%(P=0.012);蛋白水平较对照组减低7.41%(P=0.031)。结论sIL-13Rα2在NIH-3T3细胞中对IL-13有抑制作用,提示sIL-13Rα2在治疗血吸虫病肝纤维化中具有潜在价值。

首发精神分裂症患者血浆IL-6、sIL-6R及IL-13水平研究

目的 探讨首发精神分裂症患者血浆白细胞介素 6(IL 6)、可溶性白细胞介素 6受体 (sIL6R)及白细胞介素 13(IL 13)水平的变化。方法 采用酶联免疫吸附法 (ELISA)对 30例精神分裂症患者和 28例健康对照者血浆IL 6、sIL 6R及IL 13水平进行检测。结果 精神分裂症患者血浆IL 6 [ ( 20. 18±2. 59)pg/ml]及sIL 6R[ (33. 87±16. 51)pg/ml]水平显著高于对照组 (P<0. 05),而血浆IL 13 [ (16. 15±11. 98)pg/ml]水平显著低于对照组 [ (24. 41±18. 26)pg/ml] (P<0. 05);以阴性症状为主患者的IL 6[ (21. 04±1. 72)pg/ml]及sIL 6R[ (32. 83±15. 72)pg/ml]水平均高于阳性组,其中阴性组患者IL 6显著高于阳性组[ (18. 28±3. 22)pg/ml] (P<0. 05),阴性组患者血浆IL 13[ (12. 72±9. 01)pg/ml]水平显著低于阳性组[ (19. 82±7. 83)pg/ml] (P<0. 05);未发现患者组及对照组血浆IL 6、sIL 6R及IL 13之间的相关性。结论 精神分裂症患者存在IL 6、IL 13介导的免疫功能异常,血浆IL 6水平升高、IL 13水平降低可能是阴性症状为主患者的特征性免疫学指标之一。

釜内增韧PP橡胶组分序列结构^(13)C-NMR谱数据的统计理论处理

首先用Bernoullian模型和Markov模型统计公式对10组釜内增韧PP橡胶组分(乙丙共聚物)13C-NMR谱数据进行分析比较,由其所得方差值可知,所有样品中的橡胶组分数据均不符合Bernoullian模型,而符合一级Markov模型;然后用Markov模型的统计公式计算,画出共聚物乙烯、丙烯的数量和质量分布曲线,由此可直观地比较各样品的组成分布;同时定量给出了共聚物数均和重均链段长度、链段分布指数及长链段的含量。

日本血吸虫感染鼠巨噬细胞IL-13Rα2的表达

目的检测IL-13的诱骗受体IL-13Rα2在血吸虫病巨噬细胞的表达,为从细胞水平探讨Th2型免疫性疾病分子病理机制奠定基础。方法建立日本血吸虫病鼠模型,采用免疫荧光标记法分别检测肝肉芽肿和原代巨噬细胞IL-13Rα2蛋白的表达情况。结果荧光显微镜下观察:肝肉芽肿内可见似"咖啡豆样"散在分布的IL-13Rα2免疫阳性信号,巨噬细胞膜内缘呈异常增强的环状荧光。结论巨噬细胞是IL-13Rα2阳性表达细胞,IL-13Rα2是血吸虫病重要的免疫病理调节分子。

不同热轧压下率对06Cr13/Q345R爆炸复合板微观组织和拉伸断口的影响

采用不同热轧压下率,对06Cr13/Q345R爆炸复合板进行了轧制实验。采用超景深显微镜和扫描电镜(SEM)分别对不同热轧压下率的06Cr13/Q345R爆炸+轧制复合板微观组织和拉伸断口进行了研究。结果表明:轧制后的06Cr13/Q345R爆炸复合板消除了爆炸产生的熔化区、空洞等缺陷;随着轧制压下率的增大,复合板的微观组织细化程度增加;热轧后,拉伸断口都是延性断裂,有非常明显的大量韧窝。

生防菌R13对水稻纹枯病病原菌的抑制作用

测定了生防菌R13对水稻纹枯病病原菌的抑菌率、菌丝的抑制作用以及对菌核萌发与形成的影响。结果表明:生防菌R13对水稻纹枯病病原菌具有一定的抑制作用,抑菌率为67.8%,可以导致正常的纹枯病菌丝体发生扭曲、变形、原生质外溢,经生防菌R13处理后的菌丝萌发指数为34.6,并且明显延迟了菌核的形成时间。

正火热处理对06Cr13/Q345R复合钢板组织和性能的影响

重点研究了正火热处理对06Cr13/Q345R不锈钢复合钢板组织和性能的影响。试验结果表明:06Cr13/Q345R不锈钢复合钢板正火热处理后复层06Cr13晶界有大量碳化物析出,塑性降低。