Effects of septal nucleus lesion on dopamine D_2 receptor expression in the prefrontal lobe, striatum, and brainstem in a rat model of schizophrenia

BACKGROUND： It has been demonstrated that the septal nucleus is involved in the pathogenesis of schizophrenia. Based on autopsies of schizophrenia patients, studies have shown a reduced number of septal nucleus neurons and glia. In addition, experimental rat models of schizophrenia have shown increased dopamine receptor D2 binding sites in the basal ganglia, septal nuclei, and substantia nigra. Previous studies have demonstrated that the septal nucleus modulates dopamine metabolic disorder and dopamine D2 receptor balance. OBJECTIVE： Dopamine D2 receptor expression in a rat model of schizophrenia, combined with antipsychotic drugs, was analyzed in the prefrontal lobe, striatum, and brainstem. In situ hybridization was used to observe the effects of stereotactic septal nucleus lesions on dopamine D2 receptor expression in the brains of methylamphetamine-treated rats. DESIGN, TIME AND SETTING： A randomized, controlled, animal experiment was performed in the Laboratory of General Institute of Psychosurgery, Third Hospital of Chinese PLA from November 2005 to June 2006. MATERIALS： A total of 120 healthy, adult Sprague Dawley rats, weighing approximately 200 g, were included. Methylamphetamine （Sigma, USA） and an in situ hybridization detection kit for dopamine D2 receptor （Boster, China） were also used for this study. METHODS： All rats were randomly allocated to the following 4 groups, with 30 rats in each group： normal control, simple administration, septal nucleus lesion, and sham-operated groups. In the normal control group, rats were not administered or lesioned. In the remaining 3 groups, rats were intraperitoneally administered 10 mg/kg methylamphetamine, once per day, for 15 successive days to establish a schizophrenia model. Following successful model establishment, rats from the septal nucleus lesion group were subjected to stereotactic septal nucleus lesions. The cranial bone was exposed in rats from the sham-operated group, and the septal nucleus was not lesioned. MAIN OUTCOME MEASURES： At 7 days post-surgery, dopamine D2 receptor expression in the prefrontal lobe, striatum, and brainstem were detected by in situ hybridization. RESULTS： Dopamine D2 receptor expression in the rat prefrontal lobe, striatum, and brainstem was significantly higher in the simple administration group and sham-operated group, compared with the normal control group （P 〈 0.01）. In the septal nucleus lesion group, dopamine D2 receptor expression was significantly less than the simple administration and sham-operated groups, （P 〈 0.01）. There was no significant difference in dopamine D2 receptor expression between the simple administration and sham-operated groups （P 〉 0.05）. CONCLUSION： Septal nucleus lesions reduce dopamine D2 receptor expression in the prefrontal lobe, striatum, and brainstem in a rat model of schizophrenia, indicating that the septal nucleus modulates dopamine D2 receptor expression.

Modeling of Dopamine D2 Receptor and its Agonist DOCK Analyses

A model of transmembrane helices of dopamine D2 receptor was constructed using the X ray coordinates of bacteriorhodopsin (BR) as a template. Based on the results from the model and the site directed mutagenesis experience, the binding pocket, including nine amino acid residues beside indispensable Asp86, Ser141 and Ser144 residues, was defined. In order to testify the 3D structure of dopamine D2 receptor and specially test the binding sites, two sets of D2 receptor agonists (one was rigid and the other flexible) were selected for docking. A good result of correlation between logIC 50 and binding energy E b indicates that the predicted model is reliable for the investigation of the receptor ligand interaction and design of new active molecules.

Effects of Ovariectomy and 17<i>β</i>-Estradiol Replacement on Dopamine D2 Receptors in Female Rats: Consequences on Sucrose, Alcohol, Water Intakes and Body Weight

Background: Mechanisms underlying overeating-induced obesity in post-menopausal woman include functional lack of 17β-estradiol dysregulating dopamine D2 receptors, thereby inducing food addiction, glucose craving or alcohol dependence through reward circuitry. This study aimed at further understanding 17β-estradiol and dopamine D2 receptors interferences in the etiology of woman obesity. Method: Seventy-two Wistar female rats weighing 200 - 205 g, individually-housed, were divided into non-ovariectomized control (C = 6 groups) and ovariectomized rats (OVX = 6 groups) which were concurrently subjected to the following treatments: Non-drug-treated (DMSO vehicle), 17β-estradiol (E2, 5 μg/kg, s.c.), sulpiride (SUL, 20 mg/kg, i.p.), bromocriptine (BR, 0.1 mg/kg, i.p.), E2 + SUL or E2 + BR, designating the 6 constitutive groups of either control or ovariectomy. Within each experimental group, consumption of different solutions (10% alcohol, 10% sucrose and water) as well as food intake and body weight were daily measured, for 10 consecutive days. Results: This study indicated that D2S was a specific inducer of alcohol and food intakes, but reduced sugar consumption. In addition, 17β- estradiol regulated the body weight set point, modulating D2S functions towards increased food intake at lower weights and decreased food intake at higher weights. D2S met the slow genomic actions induced by 17β-estradiol. Conversely, D2L inhibited alcohol and food intakes, but induced specifically sugar consumption, thereby regulating blood glucose levels and promoting energy expenditure in reducing body weight. Indeed, 17β-estradiol exerted a tonic inhibition on D2L which was released by OVX, exacerbating sugar intake and increasing body weight. D2L mediated the rapid metabolic effects of 17β-estradiol. Conclusion: Our results supported physiological data reporting that activation of the mostly expressed presynaptically D2S-class autoreceptors decreased dopamine release stimulating food intake, whereas activation of the predominantly postsynaptic isoform D2L receptors increased dopamine activity inhibiting food intake. Our studies indicated that 17β-estradiol acted on the two types of D2 receptors showing opposite functions to equilibrate energy intake vs. expenditure for weight set point regulation. Our data also supported biochemical findings reporting that 17β-estradiol induced D2 genes transcriptional regulation, thereby involving both types of D2 receptors in the etiology of obesity. The combined dysregulated effects of D2L and D2S receptors, as 17β-estradiol was lacking, would be causal factors underlying the etiology of obesity.

Effects of endogenous dopamine induced by low concentration atropine eye drops on choroidal neovascularization in high myopia mice

AIM:To evaluate effects of endogenous dopamine induced by low concentration atropine eye drops on choroidal neovascularization(CNV)in high myopia mice.METHODS:The C57BL/6J mice were deprived of the right eye for 4wk,and the high myopia was diagnosed by optometry,the diopter was less than-6.00 D,and CNV was induced by 532 nm laser.The changes of dopamine D1 receptor(DRD1),dopamine D2 receptor(DRD2),and vascular endothelial growth factor A(VEGFA)were detected by Western blot technology at 0.5,1,2h,and 7d after 0.01%,0.05%,and 0.1%atropine eye drops,respectively,the area of CNV was measured.RESULTS:Significant increases were observed on the expression of DRD2 in mouse high myopia model at 0.5,1,2h,7d with 0.05%and 0.1%atropine eye drops(P<0.05).Significant decreases were observed on the expression of DRD1 and VEGFA in mouse high myopia model at 0.5,1,2h,7d with 0.05%and 0.1%atropine eye drops(P<0.05).The area of CNV induced by laser in the drug-treated group was significantly smaller than that in the control group,and the higher the concentration,the more significant the inhibitory effect(P<0.05).CONCLUSION:The 0.01%,0.05%,0.1%atropine eye drops can decrease the level of VEGFA and inhibit high myopia CNV indirectly by up-regulating the level of DRD2 and down-regulating the level of DRD1,and the effect of 0.05%and 0.1%atropine eye drops is more significant.

Cell-type specific examination of central amygdala dopamine receptor 2 expressing neurons as a translational target for pharmacological enhancement of extinction

Behavioral and molecular characterization of cell-type specific populations governing fear learning and behavior is a promising avenue for the rational identification of potential therapeutics for fear-related disorders.Identification of cell-type specific changes in neuronal translation following fear learning allows for targeted pharmacological intervention during fear extinction learning,mirroring possible treatment strategies in humans.Here we identify the central amygdala(Ce A)Drd2-expressing population as a fear-supporting population that is molecularly distinct from other,previously identified fear-supporting CeA populations.Sequencing of actively translating transcripts of Drd2 neurons identifies m RNAs that are differentially regulated following fear learning including Npy5r,Rxrg,Sst5r,Fgf3,Erb B4,Fkbp14,Dlk1,Ssh3 and Adora2a.Direct pharmacological manipulation of NPY5R,RXR,and ADORA2A confirms their importance in fear behavior and validates the present approach of identifying pharmacological targets for the modulation of emotional learning.

Down-regulation of dopamine D2 receptor associates with impaired reversal learning induced by morphine withdrawal

OBJECTIVE Cognitive inflexibility plays a critical role in the compulsive drug taking,a central characteristic of drug addictions,yet its underlying neurochemical mechanisms are not well understood.The present study examined the impact of morphine withdrawal on reversal learning.METHODS Reversal learning was tested in a four-choices digging task.Some brain tissues were harvested 2 h after the behavioral experiment for the further measurement.RESULTS We found that after long-term abstinence for a month from chronic morphine exposure,mice exhibited a profound reversal learning deficit.We further found that dopamine D2 receptor(D2R)system in the frontal-striatal circuit is significantly down-regulated,at both receptor and downstream signals levels.Subsequent pharmacological experiments demonstrated that aripiprazole,a D2R partial agonist,prevented the D2R downregulation and rescued the reversal learning deficit.CONCLUSION Together,our findings provide valuable insights into the causal relationship between D2R system in the frontal-striatal circuit and the cognitive inflexibility caused by abused drugs and offer a promising possibility of an effective therapeutic intervention for drug addictions.

Effect of total isoflavones from pueraria lobata on the expressions of preproenkephalin, prodynorphin and D2 dopamine receptor mRNA in PC12 cells induced by MPP^+

Objective： The aim of the study was to observe the effect of total isoflavones from pueraria Iobata （TIP） on D2 dopamine receptor mRNA, preproenkephalin mRNA and prodynorphin mRNA expressions in Parkinson＇s disease （PD） model cells induced by 1-methyl-4-phenylpyridinium ion （MPP^＋）. Methods： TIP was dissolved in 0.1 M NaOH and added to the culture medium at a final concentrations of 50 mg/L, 100 mg/L and 200 mg/L. Some cells （control） were exposed to 0.001 M NaOH. TIP was added to PC12 cells 30 min prior to the administration of MPP^＋. TIP and MPP^＋ remained in the culture medium for 96 h. D2 dopamine receptor mRNA, preproenkephalin mRNA and prodynorphin mRNA expressions were assayed by real-time quantitative reverse transcription-PCR. Results： The D2 dopamine receptor mRNA and preproenkephalin mRNA expressions were up-regulated in MPP^＋ group compared with the control group, and prodynorphin mRNA expression was down-regulated in that. The D2 dopamine receptor mRNA expression being down-regulated and prodynorphin mRNA expression being up-regulated in TIP group compared with the MPP^＋ group. And there was no effect of TIP on preproenkephalin gene expression in PC12 cells induced by MPP^＋. Conclusion： The results suggest that TIP down-regulates the D2 dopamine receptor mRNA expression, up-regulates prodynorphin mRNA expression and not affects preproenkephalin gene expression in PC12 cells induced by MPP^＋.

多巴胺D_2受体TaqIA多态性与海洛因依赖行为相关性

目的 :探讨多巴胺 (DA)受体D2 亚型基因TaqIA多态性与海洛因依赖者行为之间的相关性。方法 :应用PCR -RFLP法对 6 6例海洛因依赖病人与 132例正常人D2 R基因的TaqIA多态性特征进行对照研究。以A型行为问卷 (TABPQ) [1] 测评海洛因依赖者的行为类型 ,与其TaqIA多态性特征进行相关分析。结果 :海洛因依赖组与正常对照组DRD2 基因的TaqIA多态性基因型及等位基因频率有显著性差异 (前者携带A1等位基因的频率为 0 6 1,后者携带A1等位基因的频率为 0 31,P <0 0 5 ) ,携带A1等位基因更易形成海洛因依赖者 (比值比OR :3 47,P <0 0 5 )。各种行为类型的海洛因依赖者之间 ,基因型 (TaqIA多态性 )无显著性差异 (P >0 0 5 )。结论 :多巴胺D2 受体基因的TaqIA多态性与海洛因依赖相关连。多巴胺D2 受体基因TaqIA多态性与海洛因依赖者成瘾性的形成可能相关。这种基因位点特征可能与其他候选基因及环境因素共同作用 。

吗啡依赖大鼠脑多巴胺转运蛋白及D_2受体的研究

目的 观察吗啡依赖 (MD)大鼠脑多巴胺 (DA)系统的变化。方法 采用两隔室 (C1及C2 )模型训练大鼠对吗啡产生条件性位置偏爱 ,造成MD大鼠模型 ,用DA转运蛋白 (DAT)及DAD2 受体显像剂12 5I 甲苯 3β (4 碘苯基 )托烷 2 β 羟酸酯 (β CIT)、12 5I 左旋 3 碘 2 羟基 6 甲氧基 N[(1 乙基 2 吡咯烷 )甲基 ]苯酰胺 (IBZM)脑放射自显影、脑内放射性分布观察MD及对照组大鼠脑内D2 受体及DAT的变化。结果 条件性位置偏爱实验自第 6d后MD组大鼠由C1进入C2时间平均 (0 84±0 5 0 )min ,与对照组 (2 .40± 1.10 )min比较差异有显著性 (P <0 .0 5 ) ;放射自显影图像分析示 :12 5I β CITMD组纹状体 (ST) /小脑 (CB)及伏隔核 (NAC) /CB摄取比值分别为 4.76± 0 .92、2 .72± 0 96 ,与对照组 (5 .92± 0 .6 7、4.16± 0 .5 6 )比较差异有显著性 (P <0 .0 5 ) ;12 5I IBZM在MD组的ST/CB和NAC/CB摄取比值分别为 4.11± 0 .5 6、2 .6 4± 0 .2 5 ,明显低于对照组 (5 .43± 0 .74、3.49± 0 .6 5 ,P <0 0 5 ) ,脑内分布研究 (%ID/g脑组织湿重 )也证实MD组12 5I β CIT、12 5I IBZMST/CB摄取比值分别比对照组降低(2 1 6 8± 11.11) %和 (18.6 9± 9.97) %。结论 应用12 5I β CIT、12 5I IBZM能够敏感地反映MD?

多巴胺D_2受体显像剂Epidepride的合成及其^(131)I标记

以 3-甲氧基水杨酸为原料合成了 Epidepride[S- ( - ) - N- [( 1-乙基 - 2 -吡咯烷基 )甲基 ]- 5-碘 - 2 ,3-二甲氧基苯甲酰胺 ]及其标记前体 ( S- ( - ) - 5- (三正丁基锡 ) - N- [( 1-乙基 - 2 -吡咯烷基 )甲基 ]2 ,3-二甲氧基苯甲酰胺 ) ,并采用双氧水法对标记前体进行 131I标记 ,获得 131I- epidepride,标记率和放化纯度均大于 95%。13 1I- epidepride溶液体外稳定性好 ,4℃放置 15d放化纯度仍大于 90 %。131I- epide-pride与 D2 受体亲和力高 ,大鼠脑内纹状体与小脑的摄取比在 32 0 min时高达 2 37;在脑内纹状体的吸收可被 Spiperone完全阻断。因此 ,131I- epidepride有望成为多巴胺 D2 受体 SPECT显像剂。

端粒酶永生化的人单克隆神经前体细胞系诱导表达多巴胺D_2受体

目的 :检测人神经前体细胞系HNG12 10 E能否诱导表达多巴胺D2 受体mRNA和受体蛋白 ,表达的受体是否有生理功能。方法 :细胞因子诱导分化 ,RT PCR和免疫荧光染色检测D2 的表达 ;Fluo 3测定多巴胺刺激产生的胞浆Ca2 + 。结果 :RT PCR显示D2 mRNA诱导后阳性 ,免疫荧光结果显示诱导后D2 受体蛋白在细胞膜表面阳性 ,Fluo3法测定胞浆Ca2 + ,结果显示诱导后的细胞对 5mmol·L-1多巴胺递质反应使胞浆Ca2 + 快速上升。结论 :从mRNA、蛋白和生理功能 3个层次均证明HNG12 10 E细胞系诱导后表达D2 。

多巴胺D_2受体基因启动子A-241G多态性在精神分裂症家系中的连锁不平衡传递

目的 :探讨多巴胺D2 受体基因 (dopamineD2 receptor,DRD2 )启动子A 2 41G多态性与精神分裂症的关系。方法 :采集 10 1个家系 ,每家有 2名或 2名以上符合ICD 10精神分裂症诊断标准患病同胞且父母存活。对DRD2启动子的A 2 41G多态性进行检测。结果 :(1)DRD2启动子的A 2 41G等位基因频度和基因型频度在父母组、非患病同胞组和患病同胞组之间差异无显著性 ,在 3组不同性别之间以及在精神分裂症不同亚型之间基因型频度和等位基因频度的分布差异亦无显著性 ;(2 )传递不平衡检验发现在患病同胞 (χ2 =0 .94,P >0 .0 5 ,OR =0 .83,95 %可信区间 0 .5 7～ 1.2 1)中未表现传递不平衡性 ,而在非患病同胞 (χ2 =6 .76 ,P <0 .0 1,OR =3 .17,95 %可信区间 0 .41～ 2 4.71)中存在传递不平衡性 ,其中 2 41A等位基因在非患病同胞中传递较多 ;(3)基因型与妄想总分、幻觉总分、思维形式障碍、情感障碍、精神性失语及症状持续时间等临床特征相关。结论 :DRD2启动子的A 2

多巴胺D_2受体TaqI A多态性与海洛因渴求程度的关联分析

目的 探讨多巴胺D2 受体TaqIA多态性与线索诱发海洛因渴求程度的关系。 方法 380名海洛因依赖者接受环境诱发渴求实验 ,用PCR RFLP技术检测DRD2 受体TaqIA多态性 ,比较不同基因型与线索暴露前后渴求程度的关系。结果 强制戒毒被试者基因型与暴露前后渴求程度未见显示差异 (P >0 0 5 )。自愿戒断被试者基因型与诱发后渴求分值、暴露前后渴求分差值的差异有显著性 (F =4 5 2 3,P =0 0 12 ;F =3 936 ,P =0 0 2 1) ,A1/A1基因型被试者暴露后渴求程度高于A2 /A2 (P =0 0 2 7,P =0 0 19)和A1/A2 (P =0 0 32 ,P =0 0 35 )被试者。三者基因型在成瘾、加量和海洛因使用时间差异上有显著性 (P =0 0 14 ,P =0 0 0 1,P =0 0 0 4 )。A1/A1基因型个体成瘾时间和加量时间小于A2 /A2 (P =0 0 0 7,P =0 0 0 1)和A1/A2 (P =0 0 2 3,P =0 0 0 1)基因型个体 ,但吸毒时间大于A1/A2 (P =0 0 0 3)和A2 /A2 (P =0 0 0 2 )基因型个体。结论 DRD2 受体基因TaqIA多态性可能与环境诱发海洛因渴求程度易感性和成瘾、加量及毒品使用时间有关 ,A2 + (A2 /A2 ,A1/A2 )基因型可能在海洛因依赖中起保护作用 ,而A2 -(A1/A1)基因型则可能具有促进作用。

不同证候的注意缺陷多动障碍患儿多巴胺D_2受体基因携带情况检测

注意缺陷多动障碍（ａｔｅｎｔｉｏｎｄｅｆｉｃｉｔｈｙｐｅｒｃａｔｉｖｉｔｙｄｉｓｏｒｄｅｒ，ＡＤＨＤ）是常见的儿童行为障碍，目前病因尚未明确。国外近年由于分子生物学方法的介入，发现多巴胺Ｄ２受体ＴａｑＩＡ１等位基因与本病相关。通过对广州市城镇学龄儿童多巴胺Ｄ２受体基因ＴａｑＩＡ多态性的检测，支持Ａ１等位基因与本病的关系（Ｐ＝０．００６５２０）；并发现该基因与中医辨证的“肾虚肝亢”证候关系更为密切（Ｐ＝０．０００１２２），而“心脾不足”证候则与正常对照组间无显著性差异（Ｐ＝０．９１０９５２），因而在基因水平上为ＡＤＨＤ的中医辨证提供了参考思路。

多巴胺D_2受体显像剂^(125)I-IBZM的合成与标记

合成了标记前体Ｓ－（－）－２－羟基－６－甲氧基－Ｎ－［（１－乙基－２－吡咯烷基）甲基］苯甲酰胺（Ｓ－（－）－ＢＺＭ）。光谱数据与结构相符。以Ｓ－（－）－ＢＺＭ为前体，用１２５Ｉ－ＮａＩ标记，成功地制备了Ｓ－（－）－３－１２５Ｉ－２－羟基－６－甲氧基－Ｎ－［（１－乙基－２－吡咯烷基）甲基］苯甲酰胺（Ｓ－１２５Ｉ－ＩＢＺＭ）。标记率大于８０％，放射化学纯度大于９０％，整个制备过程仅需４５ｍｉｎ，利于药盒化生产。

多巴胺D_2受体启动子区域基因多态性与抽动-秽语综合征的关联分析

目的 :探讨抽动 秽语综合征 (TS)与多巴胺D2 受体启动子区域 (DRD2P)多态性的关系 .方法 :应用聚合酶链反应 限制性片断长度多态性技术对 2 4例患儿和 30例正常对照进行DRD2P基因 1 4 1CDel/Ins多态性和TS的关联性分析 .结果 :共检出 2种基因型 :纯合子 1 4 1CIns/Ins(1 6 0bp ,1 4 4bp)与杂合子 1 4 1CDel/Ins(30 4bp ,1 6 0bp ,1 4 4bp) ,未检出纯合子 1 4 1CDel/Del(30 4bp ,30 4bp) .病例组 1 4 1CDel/Ins多态性的基因型频率与对照组的差异无显著性 (χ2 =0 .0 93,ν=2 ,P >0 .0 5 ) ;等位基因频率比较也无显著性差异 (χ2 =0 .0 6 0 ,ν=1 ,P >0 .0 5 ) .结论 :抽动 秽语综合征与DRD2P基因 1 4

多巴胺D_2受体配体的合成及^(99m)Tc标记(Ⅰ)——悬挂式设计

以多巴胺D2 受体配体Cl ABZM为前体 ,合成了末端带有巯基的单齿化合物 ,光谱数据与结构相符 .用配体交换法与 3 硫杂 1,5 戊二硫醇共同配位合成了“3+ 1”型混配螯合物 ,对影响标记率的诸多因素如 pH值、温度、配体用量及反应时间等进行了优化 ,得到最佳标记条件 ,标记率大于 85%

多巴胺D_2受体基因与迟发性运动障碍关联研究

目的 探讨DRD2 基因TaqI多态性的分布与迟发性运动障碍 (TD)的关联性。 方法 应用聚合酶链反应 限制性片段长度多态的方法 ,检测 10 0例精神分裂症伴TD患者、6 0例无TD患者和10 2名正常人DRD2 基因TaqI多态性 ,比较各组等位基因和基因型频率分布的差异。结果 经吻合度检验 ,精神分裂症伴有TD组、无TD组和正常对照组DRD2 基因各基因型的分布均符合Hardy Wein berg平衡法则 (χ2 =0 2 4 2 ,0 2 0 8,0 0 0 2 ,υ均 =1,P均 >0 0 5 ) ;经比较 ,显示各基因型及等位基因在各组间分布无显著性差异 (经Z检验 ,υ均 =1,P均 >0 0 5 ) ;TD患者DRD2 基因多态分布在不同性别之间无显著性差异 (P >0 0 5 ) ;在TD组中 ,基因型频数及等位基因频数与病程、服药时间、药物、剂量和AIM评分无显著性意义 (P >0 0 5 )。结论 DRD2 基因TaqI多态性可能与TD的发生无关联性。

杏仁核和扣带回联合毁损对MAP大鼠脑内多巴胺D_2受体的影响

目的探讨联合毁损杏仁核和扣带回对甲基苯丙胺(M AP)大鼠脑内边缘区多巴胺D2受体表达的影响。方法40只SD大鼠随机分为对照组、M AP组、M AP+毁损组和M AP+假毁损组,每组各10只;采用经腹腔注射M AP制备精神分裂症M AP模型,立体定向-射频毁损杏仁核和扣带回,免疫组织化学ABC法观察边缘区D2受体的表达。结果与对照组和M AP+损毁组比较,M AP组及M AP+假毁损组大鼠边缘区D2受体表达有显著性差异(P<0.01);M AP+毁损组大鼠边缘区D2受体阳性细胞率与对照组比较差异无显著性(P>0.05)。结论杏仁核和扣带回的联合毁损可抑制使用M A P诱发的边缘区D2受体表达的亢进。

杏仁核毁损对甲基苯丙胺精神分裂症大鼠边缘区多巴胺D_2受体的影响

目的探讨立体定向杏仁核毁损对甲基苯丙胺(methamphetamine,MAP)精神分裂症大鼠脑内边缘区多巴胺D2受体表达的影响。方法40只SD大鼠随机分为对照组、模型组、假手术组和手术组,每组各10只;采用经腹腔注射MAP制备精神分裂症MAP模型,立体定向-射频毁损杏仁核,原位杂交法观察边缘区多巴胺D2受体的表达。结果与对照组比较,模型组及假手术组大鼠边缘区多巴胺D2受体表达有非常显著性差异(P<0.01);手术组大鼠边缘区多巴胺DA受体阳性细胞数目与对照组比较差异无显著性(P<0.01)。结论杏仁核毁损可以抑制使用MAP而诱发的边缘区D2表达的亢进。