Monoclonal antibody targeting mu-opioid receptor attenuates morphine tolerance via enhancing morphine-induced receptor endocytosis

Morphine is a frequently used analgesic that activates the mu-opioid receptor(MOR),which has prominent side effects of tolerance.Although the inefficiency of morphine in inducing the endocytosis of MOR underlies the development of morphine tolerance,currently,there is no effective therapy to treat morphine tolerance.In the current study,we aimed to develop a monoclonal antibody(mAb)precisely targeting MOR and to determine its therapeutic efficacy on morphine tolerance and the underlying molecular mechanisms.We successfully prepared a mAb targeting MOR,named 3A5C7,by hybridoma technique using a strategy of deoxyribonucleic acid immunization combined with cell immunization,and identified it as an immunoglobulin G mAb with high specificity and affinity for MOR and binding ability to antigens with spatial conformation.Treatment of two cell lines,HEK293T and SH-SY5Y,with 3A5C7 enhanced morphine-induced MOR endocytosis via a G protein-coupled receptor kinase 2(GRK2)/b-arrestin2-dependent mechanism,as demonstrated by immunofluorescence staining,flow cytometry,Western blotting,coimmunoprecipitation,and small interfering ribonucleic acid(siRNA)-based knockdown.This mAb also allowed MOR recycling from cytoplasm to plasma membrane and attenuated morphine-induced phosphorylation of MOR.We established an in vitro morphine tolerance model using differentiated SH-SY5Y cells induced by retinoic acid.Western blot,enzyme-linked immunosorbent assays,and siRNA-based knockdown revealed that 3A5C7 mAb diminished hyperactivation of adenylate cyclase,the in vitro biomarker of morphine tolerance,via the GRK2/b-arrestin2 pathway.Furthermore,in vivo hotplate test demonstrated that chronic intrathecal administration of 3A5C7 significantly alleviated morphine tolerance in mice,and withdrawal jumping test revealed that both chronic and acute 3A5C7 intrathecal administration attenuated morphine dependence.Finally,intrathecal electroporation of silencing short hairpin RNA illustrated that the in vivo anti-tolerance and anti-dependence efficacy of 3A5C7 was mediated by enhanced morphine-induced MOR endocytosis via GRK2/b-arrestin2 pathway.Collectively,our study provided a therapeutic mAb,3A5C7,targeting MOR to treat morphine tolerance,mediated by enhancing morphine-induced MOR endocytosis.The mAb 3A5C7 demonstrates promising translational value to treat clinical morphine tolerance.

Dopamine D₁- and D₂-Receptors in Immunostimulation under Activation of Mu-Opioid Receptors in Mice with Different Psychoemotional States

The purpose of the present study was to analyze the effect of activation of mu-opioid receptors (mu-OR) on the immune response under blockade of postsynaptic D1-and D2-receptors in mice of the C57BL/6J strain displaying either aggressive or depressive-like behaviors in the social conflict model. It is shown that activation of activation of mu-OR with a highly selective agonist DAGO (100 μg/kg) increased significantly IgM-immune response not only in C57BL/6J mice with an unchanged psychoemotional state but also in mice displaying aggressive or depressive-like behaviors in the social stress model (10 days of agonistic confrontations). Selective blockade of DA receptors of the D1-type with SCH-23390 (1.0 mg/kg with DAGO administration) caused a more pronounced elevation of IgM-immune response than DAGO alone while DAGO effect was completely blocked by prior administration of D2-receptor antagonist haloperidol (1.0 mg/kg). At the same time, both SCH-23390 and haloperidol prevented the immune response increase induced by DAGO injection in mice engaged in aggressive or depressive-like behaviors. Thus, in animals not subjected to social stress DAGO-induced immunostimulation is provided only by D2-receptors, whereas in animals with altered psychoemotional state mu-opioid immunostimulation is mediated by both types of DA receptors—D1 and D2. These data provide evidence for different impacts of the main subtypes of DA receptors in the mediation of immunomodulating effects of mu-opioid system under normal and stressful conditions.

Expression of mu-opioid receptors in human chronic inflamed knee joint synovium tissue

Objective: To examine the changes of mu-opioid receptors (MORs) expression in human chronic inflamed knee joint synovium tissue. Methods:Knee joint synovium tissues were taken from 21 patients with chronic arthritis (inflamed group) and 6 fresh bodies with normal knee joints (control group). And the expression of MORs was detected by using immunohistochemistry. flow cytometry(FCM) and reverse-transcription polymerase chain reaction (RT-PCR). Results: The expression of MORs in the inflamed group was significantly higher than that in the normal group by using the 3 techniques(P<0. 05). Conclusion: Chronic inflammation enhances the up-regulation of MORs in human knee joint synovium tissue.

Bispecific sigma-1 receptor antagonism and mu-opioid receptor partial agonism:WLB-73502,an analgesic with improved efficacy and safety profile compared to strong opioids

Opioids are the most effective painkillers,but their benefit-risk balance often hinder their therapeutic use.WLB-73502 is a dual,bispecific compound that binds sigma-1(S1R)and mu-opioid(MOR)receptors.WLB-73502 is an antagonist at the S1R.It behaved as a partial MOR agonist at the G-protein pathway and produced no/unsignificantβ-arrestin-2 recruitment,thus demonstrating low intrinsic efficacy on MOR at both signalling pathways.Despite its partial MOR agonism,WLB-73502exerted full antinociceptive efficacy,with potency superior to morphine and similar to oxycodone against nociceptive,inflammatory and osteoarthritis pain,and superior to both morphine and oxycodone against neuropathic pain.WLB-73502 crosses the blood-brain barrier and binds brain S1R and MOR to an extent consistent with its antinociceptive effect.Contrary to morphine and oxycodone,tolerance to its antinociceptive effect did not develop after repeated 4-week administration.Also,contrary to opioid comparators,WLB-73502 did not inhibit gastrointestinal transit or respiratory function in rats at doses inducing full efficacy,and it was devoid of proemetic effect(retching and vomiting)in ferrets at potentially effective doses.WLB-73502 benefits from its bivalent S1R antagonist and partial MOR agonist nature to provide an improved antinociceptive and safety profile respect to strong opioid therapy.

Anti-nociceptive Effect of Patchouli Alcohol: Involving Attenuation of Cyclooxygenase 2 and Modulation of Mu-Opioid Receptor

Objective: To explore the anti-nociceptive effect of patchouli alcohol(PA), the essential oil isolated from Pogostemon cablin(Blanco) Bent, and determine the mechanism in molecular levels. Methods: The acetic acid-induced writhing test and formalin-induced plantar injection test in mice were employed to con?rm the effect in vivo. Intracellular calcium ion was imaged to verify PA on mu-opioid receptor(MOR). Cyclooxygenase 2(COX2)and MOR of mouse brain were expressed for determination of PA’s target. Cellular experiments were carried out to find out COX2 and MOR expression induced by PA. Results: PA significantly reduced latency period of visceral pain and writhing induced by acetic acid saline solution(P<0.01) and allodynia after intra-plantar formalin(P<0.01) in mice. PA also up-regulated COX2 mRNA and protein(P<0.05) with a down-regulation of MOR(P<0.05) both in in vivo and in vitro experiments, which devote to the analgesic effect of PA. A decrease in the intracellular calcium level(P<0.05) induced by PA may play an important role in its anti-nociceptive effect.PA showed the characters of enhancing the MOR expression and reducing the intracellular calcium ion similar to opioid effect. Conclusions: Both COX2 and MOR are involved in the mechanism of PA’s anti-nociceptive effect,and the up-regulation of the receptor expression and the inhibition of intracellular calcium are a new perspective to PA’s effect on MOR.

Mu-Opioid Receptors Expressed in Glutamatergic Neurons are Essential for Morphine Withdrawal

Although opioids still remain the most powerful pain-killers,the chronic use of opioid analgesics is largely limited by their numerous side-effects,including opioid dependence.However,the mechanism underlying this dependence is largely unknown.In this study,we used the withdrawal symptoms precipitated by naloxone to characterize opioid dependence in mice.We determined the functional role of mu-opioid receptors(MORs)expressed in different subpopulations of neurons in the development of morphine withdrawal.We found that conditional deletion of MORs from glutamatergic neurons expressing vesicular glutamate transporter 2(Vglut2^+)largely eliminated the naloxone-precipitated withdrawal symptoms.In contrast,conditional deletion of MORs expressed in GABAergic neurons had a limited effect on morphine withdrawal.Consistently,mice with MORs deleted from Vglut2^+glutamatergic neurons also showed no morphine-induced locomotor hyperactivity.Furthermore,morphine withdrawal and morphine-induced hyperactivity were not significantly affected by conditional knockout of MORs from dorsal spinal neurons.Taken together,our data indicate that the development of morphine withdrawal is largely mediated by MORs expressed in Vglut2^+glutamatergic neurons.

RNA interference targeting mu-opioid receptors reverses the inhibition of fentanyl on glucose-evoked insulin release of rat islets

Background Mu opioid receptor plays an important role in many physiological functions. Fentanyl is a widely used opioid receptor agonist for analgesia. This study was conducted to test the role of mu-opioid receptor on insulin release by determining whether fentanyl affected insulin release from freshly isolated rat pancreatic islets and if small interfering RNAs （siRNA） targeting mu-opioid receptor in the islets could knock down mu-opioid receptor expression.Methods Islets were isolated from ripe SD rats＇ pancreas by common bile duct intraductal collagenase V digestion and purified by discontinuous Ficoll density gradient centrifugation. The siRNA knock-down of mu-opioid receptor mRNA and protein in islet cells was analyzed by semi-quantitative real time-PCR and Western blotting. After siRNA-transfection for 48 hours, the islets were co-cultured with fentanyl as follows： 0 ng/ml, 3 ng/ml and 30 ng/ml for 48 hours. Then glucose-evoked insulin release was performed. As a control, the insulin release was also analyzed in islets without siRNA-trasfection after being co-cultured with fentanyl for 48 hours.Results After 48 hours of transfections, specific siRNA targeting of mu-opioid receptors produced significant reduction of mu-opioid receptor mRNA and protein （P ＜0.01）. Fentanyl significantly inhibited glucose-evoked insulin release in islets in a concentration dependent manner （P ＜0.01）. But after siRNA-transfection for 48 hours, the inhibition on glucose-evoked insulin reiease was reversed （P ＜0.01）.Conclusions RNA interference specifically reduces mu-opioid receptor mRNA and protein expression, leading to reversal of the fentanyl-induced inhibition on glucose-evoked insulin release of rat islets. The activation of opioid receptor induced by fentanyl functions to inhibit insulin release. The use of RNAi presents a promising tool for future research in diabetic mechanisms and a novel therapy for diabetes.

基于μ阿片受体羧基端^(375)STANT^(379)磷酸化位点的多肽干预对吗啡介导的受体下游信号通路的影响

目的探讨基于μ阿片受体(MOR)羧基端^(375)STANT^(379)磷酸化位点的多肽TAT-Q368-T379干预,对μ阿片受体下游信号通路的影响。方法将HA-MOR质粒与pGloSensorTM-22F质粒共转染的HEK-293细胞分为空白组(A组)、DAMGO组(B组)、吗啡组(C组)、0.5×10^(-5)mol/L多肽TAT-Q368-T379与吗啡联用组(D组)、10-5mol/L多肽TAT-Q368-T379与吗啡联用组(E组)、2×10^(-5)mol/L多肽TAT-Q368-T379与吗啡联用组(F组),通过GloSensor cAMP生物传感器测定各组细胞中的cAMP含量。将MOR-C端标记Nanoluc的质粒以及β-arrestin2-N端标记EYFP的质粒共转染完成的HEK-293细胞分为空白组(G组)、DAMGO组(H组)、吗啡组(I组)、10^(-5)mol/L多肽TAT-Q368-T379与吗啡联用组(J组)、3×10^(-5)mol/L Cmpd101与吗啡联用组(K组),通过蛋白质相互作用分析法测定各组细胞MOR激动后对β-arrestin2的募集效应。将HA-MOR质粒转染完成的HEK-293细胞分为空白组(L组)、吗啡组(M组)、10^(-5)mol/L多肽TAT-Q368-T379与吗啡联用组(N组)以及3×10^(-5)mol/L Cmpd101与吗啡联用组(O组),通过细胞免疫荧光染色法检测各组细胞的受体平均荧光强度。结果GloSensor cAMP生物传感器检测结果显示,C~F组细胞EC_(50)值差异有显著性(F=13.12,P<0.05),其中D、E、F组EC_(50)值较C组均显著减小(P<0.05)。蛋白质相互作用分析法分析显示,I~K组细胞E_(max)值差异有显著性(F=185.95,P<0.05),其中J、K组E_(max)值较I组均显著减小(P<0.01)。细胞免疫荧光染色法染色结果显示,L~O组细胞表面受体荧光强度比较差异有显著性(F=17.46,P<0.05),其中与M组比较,N、O组细胞表面受体荧光强度均显著增高(P<0.01)。结论基于MOR羧基端^(375)STANT^(379)磷酸化位点设计的多肽TAT-Q368-T379可有效增强吗啡介导的MOR下游G蛋白信号通路的激活,减少吗啡介导的β-arrestin2招募,从而减少由吗啡介导的MOR的内吞。

不同剂量喷他佐辛抑制吗啡的镇痛作用

目的:研究不同剂量喷他佐辛对吗啡镇痛效果的影响及可能机制。方法:60只C57BL/6J小鼠随机分为10组(n=6),其中5组喷他佐辛注射前2小时预先注射生理盐水,另外5组预先注射kappa受体拮抗剂nor-BNI(10 mg/kg),随后各组同时皮下注射不同剂量喷他佐辛(0、10、30、56、100 mg/kg)和吗啡(10 mg/kg),分别于药物注射前和注射后30、60、90、120 min对小鼠进行机械痛阈(压尾试验)和热痛阈(热板试验,甩尾试验)测定,并分别计算药物时效的曲线下面积(area under curve,AUC)作为药物镇痛效应的量化指标。结果:1不同剂量喷他佐辛(0、10、30、56、100 mg/kg)在与吗啡合用后的压尾AUC分别为(244.1±19.5)、(166.5±9.6)、(146.6±8.3)、(130.7±7.8)、(124.5±10.1)(g·h);热板AUC分别为(27.9±4.0)、(24.4±1.6)、(22.8±1.6)、(23.3±2.1)、(22.7±1.2)(s·h);甩尾AUC分别为(13.1±1.9)、(12.0±1.7)、(10.4±0.8)、9.5±0.9)、(9.7±1.3)(s·h)。这提示喷他佐辛可剂量依赖地抑制吗啡的镇痛作用。2使用κ受体拮抗剂nor-BNI后,不同剂量喷他佐辛(0、10、30、56、100 mg/kg)与吗啡合用后的压尾AUC分别为(252.2±16.7)、(167.7±11.0)、(145.1±9.8)、(132.6±5.1)、(127.3±8.0)(g·h);热板AUC分别为(28.0±1.7、(25.0±1.6)、(23.0±1.2)、(22.0±1.4)、(21.2±1.3)(s·h);甩尾AUC分别为(14.4±1.8)、(11.2±1.4)、(10.2±0.8)、(9.7±0.7)、(10.1±0.8)(s·h),与上述未使用nor-BNI的各组相比差异均无统计学意义(P>0.05),结果表明kappa受体拮抗剂存在的情况下,大剂量喷他佐辛对吗啡镇痛依然存在抑制作用。结论:喷他佐辛可剂量依赖地抑制啡产生的镇痛作用,该抑制作用与kappa受体激动无关。

海马mu型阿片肽受体介导大鼠癫痫发作敏感性形成(英文)

为探讨海马mu型阿片肽受体介导癫痫发作敏感性形成的作用,实验采用微渗透泵技术,观察大鼠腹侧海马注射mu型阿片肽受体激动剂PL017(2.09、2.59、3.29 μg/μl)、拮抗剂β-funaltrexamine hydrochloride(β-FNA、0.88、1.10、1.35μg/μl)对红藻氨酸(kainic acid,KA)诱导癫痫发作的干预作用。PL017能够明显缩短癫痫发作潜伏期、增加癫痫发作级别(P<0.05),β—FNA则可显著延长癫痫发作潜伏期、降低发作级别(P<0.01);PL017和β-VNA的干预作用均表现出剂量依赖效应。结果表明,海码mu型阿片肽受体具有促进KA诱导的癫痫发作敏感性形成作用。

猪Mu阿片受体基因单核苷酸多态性分析

Mu阿片受体(简称MOR)属于G蛋白藕联受体,分布在痛觉传导区,以及与情绪和行为有关的区域,影响动物的神经反应和行为表现。该研究以长白猪、大白猪和杜洛克猪为试验材料,用8对引物对Mu阿片受体基因的5′UTR区域、整个编码区和3′UTR区域用PCR SSCP方法进行了扫描,发现5处突变基因座(GenBank登录号:AF521309)。统计结果发现基因型频率分布与品种有关,大白猪突变基因型频率显著高于长白和杜洛克,本研究推测分布上的差异可能是由于长期的选择压力造成的。

内吗啡肽对小鼠树突状细胞免疫功能的影响

目的研究内吗啡肽-1和内吗啡肽-2对小鼠骨髓来源树突状细胞表型和免疫功能的影响。方法从7～8周龄的C57BL/6J小鼠提取骨髓前体细胞培养,经CD11c免疫磁珠分选,获得纯化的树突状细胞(dendritic cells,DC)。未成熟DC用脂多糖或脂多糖+不同浓度内吗啡肽共培养,流式细胞术检测DC的表型;检测内吗啡肽对DC趋化性的影响。在DC和T淋巴细胞共培养的条件下,用氚标记胸腺嘧啶核苷(3H-TdR)参入测定的方法检测T淋巴细胞的增殖能力。结果内吗啡肽抑制DC的趋化性;与T淋巴细胞体外共培养时,经内吗啡肽-1或内吗啡肽-2处理的DC能抑制T淋巴细胞的增殖反应。上述内吗啡肽的作用都能被Mu阿片受体特异性拮抗剂CTOP翻转或部分翻转,提示内吗啡肽的作用是由Mu受体介导的。结论内吗啡肽可通过作用于Mu阿片受体,改变树突状细胞的部分免疫功能,调节免疫反应。

二氢埃托啡对大鼠脑阿片受体的结合特性

本文在大鼠脑匀浆P_2膜上,观察了二氢埃托啡(DHE)对[~3H]纳洛酮,[~3H]DPDPE和[~3H]埃托啡(预先用30nmol/L吗啡和100nmol/L DADLE阻断μ和δ受体)与阿片受体结合的抑制强度。结果表明:DHE对[~3H]纳洛酮与阿片受体结合的抑制强度远远大于对[~3H]DPDPE和[~3H]埃托啡(预先阻断μ和δ受体后)。DHE对μ,δ和κ受体的相对亲和力之比为1951:2:1,提示DHE为μ受体相对选择性配体。

μ型阿片肽受体对癫痫敏感大鼠海马NR2B表达的影响

目的探讨μ型阿片肽受体(MORs)介导大鼠癫痫敏感性形成过程中海马NMDA2B受体(NR2B)表达变化。方法红藻氨酸(KA)皮下注射建立大鼠癫痫发作模型,采用脑立体定位及微渗透泵技术,海马内微量注射MORs激动剂PL017或和拮抗剂β-FNA。7 d后通过阈下剂量KA检测大鼠癫痫发作敏感性,应用原位杂交方法观察海马CA1区锥体细胞及齿状回颗粒细胞NR2B表达变化。结果 PL017可显著增加大鼠海马CA1区锥体细胞和齿状回颗粒细胞NR2B mRNA(+)神经元数及平均灰度。β-FNA则明显降低两个脑区的NR2B mRNA(+)神经元数及平均灰度。结论 MORs介导癫痫发作敏感性形成机制与NR2B表达上调有关。

犬急性膝关节炎炎症期滑膜组织μ-阿片受体的表达

目的:观察犬急性膝关节炎炎症期滑膜组织μ-阿片受体(mu-opioid receptors,MOR)表达的变化,探讨急性炎症外周局部应用阿片类药物镇痛的可行性。方法:17只Beagle犬随机分为正常对照组(n=8)和急性感染性炎症组(n=9),取各组犬膝关节滑膜组织,采用免疫组织化学及real-ti me PCR方法检测滑膜组织MOR蛋白及mRNA的表达。结果:急性感染性炎症组犬膝关节滑膜组织MOR mRNA相对表达量明显高于正常对照组[(34.40±5.48)%vs(16.54±8.03)%],差异具有统计学意义(P<0.05)。免疫组化染色见炎症滑膜组织MOR染色阳性产物较正常对照颗粒增粗、着色加深、染色带增宽、数量增多;与正常滑膜组织相比,急性感染性炎症组滑膜组织MOR阳性细胞免疫组化指数显著增高[(323175.00±92614.94)vs(175444.10±75149.06)],差异具有统计学意义(P<0.05)。结论:犬膝关节滑膜组织中存在MOR,且在急性感染性炎症早期其表达显著增强。

瑞芬太尼对老年无痛肠镜中靶控输注丙泊酚用量的影响

目的:探讨在老年患者无痛肠镜麻醉中给予0.3μg/kg瑞芬太尼对丙泊酚TCI麻醉效能的影响。方法:将60例门诊无痛肠镜老年患者随机分为丙泊酚TCI组(P组,n=30)、瑞芬太尼复合丙泊酚TCI组(RP组,n=30)。RP组给予瑞芬太尼0.3μg/kg,P组给予生理盐水0.1ml/kg,然后按序贯法,两组依次给予不同剂量的丙泊酚计算出50%患者肠镜检查时无逃避性体动的丙泊酚血浆浓度(Cp50)。麻醉过程中连续监测患者心率(HR)、平均动脉压(MAP)、脉搏氧饱和度(SpO2)、反应熵(RE)和状态熵(SE)。结果:①RP组与P组Cp50分别为3.425μg/ml和5.011μg/ml;②与P组比较,RP组丙泊酚总量和所有患者完成检查时丙泊酚血浆浓度显著减少(P<0.01);③RP组在肠镜检查过程中RE和SE值均显著高于P组(P<0.01)。结论 :在老年患者无痛肠镜麻醉中给予0.3μg/kg瑞芬太尼可以显著减少靶控输注丙泊酚的半数有效血浆浓度,在较浅麻醉深度下就能满足肠镜检查的需要。

瑞芬太尼聚己内酯对脊髓缺血再灌注损伤兔体感诱发电位的影响

目的:观察腹主动脉内灌注Mu阿片受体(MOR)激动剂瑞芬太尼聚己内酯(REM-PCL)对脊髓缺血再灌注损伤(SCIRI)兔体感诱发电位(SEP)的影响。方法:30只健康新西兰大白兔随机分为对照组、R组和RG组,每组10只。R组和RG组采用肾下腹主动脉阻断法制备SCIRI模型,于阻断血流时经腹主动脉局部灌注REM-PCL 0.1mg/kg,RG组于REM-PCL灌注结束后再局部灌注MOR拮抗剂GSK1521498(1 mg/kg),对照组局部灌注等容量生理盐水。分别于阻断前,再灌注15、30、60 min及再灌注24 h监测血清神经特异性烯醇化酶(NSE)质量浓度和SEP;再灌注6、12和24 h进行神经行为学评分,然后于再灌注24 h取脊髓组织检测MOR mRNA和感觉神经元异常率。结果:3组血清NSE质量浓度变化、SEP变化、神经行为学评分、脊髓组织MOR mRNA表达水平和感觉神经元异常率差异均有统计学意义(P均<0.05)。RG组上述指标测值及变化趋势与对照组相似(P>0.05)。与对照组和RG组比较,再灌注期间R组血清NSE质量浓度明显较低,SEP OL延长程度较小,IPA较快恢复,神经行为学评分较低;再灌注24 h时,R组脊髓组织MOR mRNA表达水平较高,感觉神经元异常率明显较低(P<0.05)。结论:腹主动脉内灌注REM-PCL可以通过激活MOR,减轻脊髓电生理功能障碍。

大鼠中脑导水管周围灰质内GABA与阿片μ受体共存能神经元的观察

目的 观察中脑导水管周围灰质 (PAG)内是否存在γ-氨基丁酸 (GABA)与阿片μ受体 (MOR)共存神经元 .方法免疫荧光组织化学双重染色技术 ,染色结果在激光扫描共聚焦显微镜下观察 .结果 GABA阳性神经元主要见于 PAG中、尾段内侧区和腹外侧区 ,阳性神经元多散在分布并多为小型 ,中型者较少 ;散在分布的 MOR阳性神经元主要见于 PAG中、尾段的腹外侧区 ,多为中、小型神经元 ;散在并同时呈GABA和 MOR双重染色阳性的中、小型神经元主要见于PAG中、尾段的腹外侧区 .结论 PAG内有 GABA与 MOR共存的神经元 ,提示内源性阿片物质对 PAG内的

栉孔扇贝消化系统μ受体的免疫组化定位研究

采用免疫组织化学定位的方法研究了μ受体在栉孔扇贝(Chlamys farreri)消化系统的分布,结果表明:口唇上皮的大量皱褶呈μ受体阳性,少量皱褶呈μ受体强阳性,口唇结缔组织呈弱阳性或阳性;唇瓣表皮大量部位呈μ受体阳性,少量部位呈μ受体强阳性,唇瓣结缔组织呈阳性或弱阳性,结缔组织内有少量神经纤维呈阳性;胃上皮表面呈μ受体阳性,胃上皮内部呈μ受体弱阳性;肠粘膜上皮有大量μ受体阳性颗粒和弱阳性颗粒分布;直肠上皮有少量皱褶表面呈μ受体弱阳性;肝小叶中的少量细胞呈μ受体阳性,大量细胞呈μ受体强阳性,肝小叶间结缔组织呈强阳性或阳性.

μ型阿片受体与炎症性肠病

μ型阿片受体(mu opioid receptor,MOR)作为G蛋白偶联受体的成员之一,在疼痛传递、炎症过程、免疫调节等多种生理及病理反应中发挥重要作用.MOR在中枢和外周都有大量表达,在胃肠道中主要分布于肠道淋巴细胞、肠肌层及黏膜下神经元中,对肠道蠕动、分泌功能都有重要作用.一些动物实验和体外实验结果表明MOR的激动剂在治疗炎症性肠病(inflammatory bowel disease,IBD)方面具有重要的潜在价值,已经成为治疗IBD的一种新靶点.本文对MOR的功能及其与IBD的潜在联系进行了综述,为深入研究治疗IBD的新途径提供理论依据.