胰腺腺泡细胞凋亡和Fas/Fas配体表达在大鼠胰腺移植急性排斥反应中的作用

目的探讨大鼠胰腺移植后细胞凋亡的变化、Fas/Fas配体(FasL)的表达及其与急性排斥反应的关系。方法实验分为同基因移植组和异基因移植组。分别于术后第3、5、7天处死受体,取移植胰腺,应用原位末端标记法(TUNEL)检测细胞凋亡,计算凋亡指数(AI),应用免疫组织化学及Westernblot检测Fas/FasL的表达。结果细胞凋亡主要发生在胰腺腺泡细胞,同基因移植组有散在的腺泡细胞凋亡,AI在术后无明显变化,Fas/FasL表达阴性;异基因移植组在术后第3、5、7天胰腺腺泡细胞凋亡发生率逐渐增加(28.40±3.75,39.40±5.59,57.30±8.53,P<0.01),Fas/FasL表达逐渐增强,AI与急性排斥反应程度呈显著正相关(rs=0.932,P<0.01)。结论胰腺腺泡细胞凋亡和Fas/FasL表达在胰腺移植急性排斥反应中发挥重要作用,凋亡指数对胰腺移植急性排斥反应的诊断有一定的参考价值。     

腺泡细胞凋亡在大鼠胰腺移植急性排斥反应中的意义

目的：观察移植胰腺的腺泡细胞凋亡及其与急性排斥反应的关系。方法：选用SD和Wistar大鼠进行全胰十二指移植。实验分为同基因移植组（Wistar→Wistar）和异基因移植组（SD→Wistar）两组。于术后第3d、5d和7d分批处死受体，取移植胰腺标本用HE染色和原位末端标记（TUNEL）技术检测移植胰腺切片，进行排斥反应的病理学评分和计数凋亡指数（AI）。结果：发生凋亡的细胞主要是腺泡细胞，同基因移植组胰腺有散在的腺泡细胞凋亡，AI在术后无明显变化。异基因移植组胰腺腺泡细胞凋亡在术后第3d、5d和7d逐渐升高，AI与急性排斥反应的病理学评分成正相关。结论：细胞凋亡与移植胰腺急性排斥反应的严重程度显著相关，凋亡指数可作为判断移植物损伤程度的指标，对急性排斥反应的诊断有一定的参考价值。     

异基因大鼠全胰十二指肠移植急性排斥反应的病理变化

目的 观察异基因大鼠间行全胰十二指肠移植后急性排斥反应的病理变化特点。方法 实验分两组，Ⅰ组为同基因移植组，Ⅱ组为异基因移植组，术后第3，5，7，10d取移植胰腺及十二指肠行病理检查。结果 Ⅰ组移植胰腺及十二指肠后未见明显病理学改变，Ⅱ组移植胰腺术后第3d出现轻度排斥反应，第5d出现中度排斥反应，第7d发生重度排斥反应，第10d胰腺几乎完全被纤维结缔组织取代，胰腺急排斥反应首先损伤腺泡，以后累及胰腺导管，最后累及胰岛和血管，胰腺和十二指肠急性排斥反应大多同时存在，间质性排斥反应评分相同者占45%，评分不同者均以胰腺评分较高。结论 胰腺急性排斥反应首先累及外分泌组织，最后累及内分泌组织，十二指肠黏膜活检有助于确定有无胰腺急性排斥反应发生。     

小肠移植急性排斥反应中bcl-2及bax表达的意义

目的探讨bcl-2及bax的异常表达与小肠移植急性排斥反应的关系。方法选用近交系F344/N和封闭群Wistar/A大鼠建立同种异基因小肠移植模型,并随机分为同基因移植组、异基因移植组、异基因加普乐可复(FK506)治疗组和对照组,用免疫组织化学技术检测36只大鼠术后移植肠组织中bcl-2及bax在移植肠组织中的表达。结果异基因组术后第3天,bcl-2的表达显著低于对照组(P<0.05),并随着移植天数的增加,差异更加具有显著性意义(P<0.01);bax的表达与对照组比较差异无显著性意义(P>0.05);FK506治疗组bcl-2及bax表达与对照组比较,差异均无显著性意义(P>0.05)。结论移植肠组织内bcl-2表达水平可作为早期诊断急性排斥反应的一个有参考意义的指标。     

胰岛FasL基因转染对大鼠胰岛移植的影响

目的 探究胰岛细胞FasL基因转染对同种大鼠胰岛移植的影响。方法 通过磷酸钙沉淀法构建含目的基因FasL的重组腺病毒AdV-FasL,感染胰岛细胞后移植于糖尿病受者大鼠,通过RT-PCR和免疫组织化学检测移植物FasL表达,观察移植物存活情况及基因转染胰岛细胞凋亡情况。结果 单纯移植胰岛组平均存活期为（6.3±0.56）d,FasL基因转染组并未出现排斥延迟,反而排斥加速,存活期缩短至（3.4±0.24）d。FasL转染的胰岛细胞在移植后24h见FasL表达,在 48 h表达增强,AdV-5感染组及未转染组未见FasL表达。TUNEL标记见移植后FasL转染胰岛细胞凋亡。结论 尽管表达FasL的睾丸细胞与胰岛共移植可诱导活化的淋巴细胞凋亡,使胰岛移植物获得免疫豁免、存活期延长,但通过FasL基因转染使胰岛细胞直接表达FasL,引起胰岛细胞凋亡和粒细胞浸润,导致排斥加速。     

Fas配体表达对同种胰岛移植的影响

目的探究睾丸细胞FasL表达能否对共移植的胰岛移植物提供免疫豁免作用以及胰岛细胞FasL基因转染对同种胰岛移植的影响.方法将同种大鼠胰岛及睾丸细胞同时移植于糖尿病受体,重组腺病毒AdV-FasL感染胰岛细胞后移植,观察移植物存活情况、胰岛功能,并检测移植物内浸润淋巴细胞以及基因转染胰岛细胞凋亡情况.结果单纯移植胰岛组平均存活期为(6.3±0.56)?d.与胰岛细胞同时移植的睾丸细胞数增加至1×107时,存活期大于50?d(P＜0.05).表达FasL的睾丸细胞在移植物内诱导浸润淋巴细胞凋亡.FasL基因转染组出现排斥加速,存活期缩短至(3.4±0.24)?d.FasL转染的胰岛细胞在移植后24h见FasL表达,48h表达增强,移植后FasL转染胰岛细胞凋亡.结论表达FasL的睾丸细胞与胰岛同时移植可诱导活化的淋巴细胞凋亡,使胰岛移植物获得免疫豁免、存活期延长,但通过FasL基因转染使胰岛细胞直接表达FasL引起胰岛细胞凋亡和粒细胞浸润,导致排斥加速.     

大鼠肝脏移植再灌注细胞凋亡与凋亡调控的研究

目的：探讨大鼠肝脏组织再灌注后细胞凋亡及其调控机制。方法：SD大鼠132只，进行原位肝移植，取灌注保存及再灌注后的肝脏组织。采用脱氧核苷酸末端转移酶介导的缺口末端标记法和逆转录多聚酶链反应，检测肝组织中的凋亡细胞及bcl-2 mRNA、bax mRNA和Fas mRNA。结果：肝移植再灌注后，大鼠肝脏组织标本中凋亡细胞尤其明显。肝脏冷灌注保存180min时，未检测到凋亡抑制基因bcl-2的表达，但可明显检测到bax和Fas基因的表达。移植再灌注后，可检测到bax和Fas基因及凋亡抑制基因bcl-2。结论：移植再灌注肝组织中，细胞凋亡是早期细胞死亡的重要原因，其发生可能与凋亡诱导基因bax和Fas的高表达以及凋亡抑制基因bcl-2的低表达有关。     

Fas/FasL表达和细胞凋亡在大鼠同种异体肝移植免疫中的作用

目的探讨Fas和Fas配体 (fasligand ,FasL)与细胞凋亡在大鼠肝移植免疫中的作用。方法分别用免疫组织化学法及原位杂交法 ,在移植后不同的时间点 (1、3、5、7d)检测Fas FasL、Bcl 2 Bax和细胞凋亡在不同的大鼠肝移植模型中的表达情况。结果肝急性排斥组与自发耐受组相比 ,肝细胞凋亡多 ,汇管区FasL表达高而肝细胞FasL表达低 [(2 1 5± 2 5 )个细胞vs.(39 5± 0 5 )个细胞 ,P <0 0 5 ],并且Fas[(47 0± 8 1)个细胞vs.(14 5± 0 8)个细胞 ,P <0 0 5 ]和Bax[(2 1 4± 1 1)个细胞vs.(9 4± 0 9)个细胞 ,P <0 0 5 ]表达高。子代组与肝急性排斥组各指标表达类似 ,半肝组与自发耐受组各指标表达类似。在移植后第 5天 ,汇管区凋亡指数与肝细胞FasL的表达呈正相关 (r =0 76 0 ,P <0 0 1) ,而与肝细胞Fas(r =- 0 75 9,P <0 0 1)、Bax的表达呈负相关 (r =- 0 840 ,P <0 0 1)。结论肝实质细胞的凋亡与肝急性排斥反应有关 ,而其Fas、Bax的高表达可能介导了肝实质细胞凋亡的发生 ;汇管区浸润细胞凋亡与肝自发耐受有关 ,肝细胞FasL的高表达可能介导了浸润细胞凋亡的发生。     

狼疮性肾炎外周血淋巴细胞凋亡调控因子表达与中医证型的关系

目的:探讨外周血淋巴细胞(PBL)凋亡调控因子Fas、FasL、bcl-2表达在活动性狼疮性肾炎(LN)患者中的作用及其与中医证型的关系.方法:选择活动性LN患者36例进行观察,并按照中医辨证分型标准将其分为热毒炽盛型、阴虚内热型、气阴两虚型、脾肾阳虚型四型;正常健康志愿者 15例为对照.运用免疫组化法检测Fas、FasL、bcl-2在外周血淋巴细胞的表达水平.结果:活动期LN患者Fas、FasL、bcl-2表达均显著高于正常人(P<0.001),Fas、FasL与临床活动指数呈正相关(r=0.517、P<0.01;r=0.543,P<0.01),bcl-2与临床活动指数无显著相关性(r=0.09,P>0.05);三者在各中医证型之间表达皆无统计学差异.结论:Fas、FasL、bcl-2的表达升高可能导致外周血淋巴细胞凋亡异常,为SLE、LN发病机制之一;Fas、FasL表达水平可作为病情活动的指标;狼疮性肾炎中医各证型之间有着潜在、相似的发病机制.     

转染转化生长因子β1基因减轻非协调性异种心脏移植急性血管性排斥反应

目的探讨移植物局部转染转化生长因子β1(TGF-β1)基因对非协调性异种心脏移植急性血管性排斥反应(AVR)的影响。方法建立豚鼠到SD大鼠的颈部心脏移植模型,移植前受鼠接受中华眼镜蛇毒因子和环孢素A预处理,供心切取后,经冠状动脉按每克心肌组织灌注5×1010PFU携带TGF-β1基因的重组腺病毒载体进行基因转染,再移植到经过预处理的SD大鼠颈部(基因转染组),另设灌注5×1010PFU腺病毒空白载体的空白载体组和对照组。术后观察各组移植物的存活情况、移植物组织学变化情况以及移植物中CD68和CD57的表达、细胞凋亡指数、TGF-β1的表达。结果基因转染组移植物的存活时间为(95±3)h,明显长于空白载体对照组的(57±2)h和对照组的(60±2)h(P<0.01);各组移植物均呈急性血管性排斥反应的病理改变,但基因转染组较轻;基因转染组移植物组织中炎症细胞浸润数、CD68和CD57的表达量及细胞凋亡指数明显低于空白载体对照组和对照组,并能检测到外源性TGF-β1的表达。结论经冠状动脉灌注重组腺病毒载体介导的TGF-β1基因转移可减轻非协调性异种心脏移植AVR,明显延长移植物的存活时间。     

杭州健康女性定量骨超声测定原发性骨质疏松

目的 评价杭州健康女性骨超声速度(SOS)值随增龄减少和骨质疏松患病率，建立杭州地区女性骨超声速度值参考数据库。方法 定量超声法测定1208例杭州地区健康女性桡骨远端(RAD)，第3指骨近节(PLX)，第V跖骨(MTR)和胫骨中段(TIB)的超声速度值。结果 RAD、PLX、MTR和TIBSOS峰值(Peak of SOS)均出现在40-45岁，TJB的SOS峰值出现在35—40岁，此后随年龄增长而下降。绝经后妇女在绝经后早期和晚期各有1个SOS快速减少期，前见于桡骨近端，平均年减少率为2．4％，后见于胫骨中段，平均年减少率为1．8％。各部位骨SOS累积减少率随年龄增长而增加，到85岁4部位累积减少为13％-18％。60岁以后骨质疏松性症(OP)检出率为45％-70％，OP检出率以桡骨远端最高，60-70岁平均为67％，第3指骨近端次之约50％，胫骨中段最低为36％；75岁以后分别为70％，65％和45％。结论 全身各部位骨超声速度值到达峰值的年龄不同，峰值也各有差异。绝经后妇女骨超声速度值随年龄增加减少较快，应予激素和补钙治疗，桡骨远端为本地区SOS检测和OP检出的敏感部位。     

Importance of echocardiography in prognosis of surgical outcomes in cholecystitis in elderly patients

The authors propose to use more often echocardiography (EchoCG) in examination of elderly (over 60 years) of age patients with cholecystitis that permits to increase surgical activity to 92.4%. Left ventricular ejection fraction is the most informative. When this fraction is lower than 45% surgery must be recommended on vital indications only. EchoCG was used in 155 patients with cholecystitis, 131 of them were operated. 2 (1.52%) patients died due to acute cardio-vascular insufficiency and pulmonary artery thromboembolism.     

脊髓胶质细胞在小鼠骨癌痛形成中的作用

Objective To evaluate the role of gliocyte in the spinal cord in the development of bone cancer pain (BCP) in mice. Methods Forty male C3H/He mice aged 8-10 weeks weighing 18-22 g were randomly divided into 4 groups ( n = 10 each) : group I sham operation (group S) , group II BCP, group Ⅲ PBS and group IV minocyline (group M) . In group BCP, PBS and M, bone cancer pain was produced by injection of NCTC2472 fibrosarcoma cell suspension (2 x 105 cells) 10 μl into medullary cavity of calcaneus bone, while in group S, PBS solution 10 μl was injected instead of cancer cell suspension. In group PBS and M, PBS 5 μl and minocyline 5 μl (dissolved to 0.2 mmol/L in PBS)_were given IT immediately before cancer cell inoculation once a day for 11 consecutive days respectively. Mechanical pain threshold was measured at 1 d before cancer cell inoculation, and at 0, 3, 5, 7, 9 and 11d after cancer cell inoculation. Cold pain threshold was measured at 3, 7, 9 and 11d after cancer cell inoculation. The animals were killed after measurement of pain threshold and L4-6, segment of spinal cord was removed for determination of GFAP and CD11b expression by Western blot. Results Compared with group S, mechanical pain threshold was significantly increased at 3-11 d after cancer cell inoculation in group BCP and PBS, and at 3 and S d after cancer cell inoculation in group M, and cold pain threshold was significantly increased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was up-regulated in group BCP, PBS and M ( P < 0.05) . Compared with group BCP, mechanical pain threshold was significantly decreased at 3-11 d after cancer cell inoculation, cold pain threshold was significantly decreased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was down-regulated in group M ( P <0.05) . ConclusionThe activiton of gliocyte in the spinal cord is involved in the development of bone cancer pian in mice.     

脊髓胶质细胞在小鼠骨癌痛形成中的作用

Objective To evaluate the role of gliocyte in the spinal cord in the development of bone cancer pain (BCP) in mice. Methods Forty male C3H/He mice aged 8-10 weeks weighing 18-22 g were randomly divided into 4 groups ( n = 10 each) : group I sham operation (group S) , group II BCP, group Ⅲ PBS and group IV minocyline (group M) . In group BCP, PBS and M, bone cancer pain was produced by injection of NCTC2472 fibrosarcoma cell suspension (2 x 105 cells) 10 μl into medullary cavity of calcaneus bone, while in group S, PBS solution 10 μl was injected instead of cancer cell suspension. In group PBS and M, PBS 5 μl and minocyline 5 μl (dissolved to 0.2 mmol/L in PBS)_were given IT immediately before cancer cell inoculation once a day for 11 consecutive days respectively. Mechanical pain threshold was measured at 1 d before cancer cell inoculation, and at 0, 3, 5, 7, 9 and 11d after cancer cell inoculation. Cold pain threshold was measured at 3, 7, 9 and 11d after cancer cell inoculation. The animals were killed after measurement of pain threshold and L4-6, segment of spinal cord was removed for determination of GFAP and CD11b expression by Western blot. Results Compared with group S, mechanical pain threshold was significantly increased at 3-11 d after cancer cell inoculation in group BCP and PBS, and at 3 and S d after cancer cell inoculation in group M, and cold pain threshold was significantly increased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was up-regulated in group BCP, PBS and M ( P < 0.05) . Compared with group BCP, mechanical pain threshold was significantly decreased at 3-11 d after cancer cell inoculation, cold pain threshold was significantly decreased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was down-regulated in group M ( P <0.05) . ConclusionThe activiton of gliocyte in the spinal cord is involved in the development of bone cancer pian in mice.     

脊髓胶质细胞在小鼠骨癌痛形成中的作用

Objective To evaluate the role of gliocyte in the spinal cord in the development of bone cancer pain (BCP) in mice. Methods Forty male C3H/He mice aged 8-10 weeks weighing 18-22 g were randomly divided into 4 groups ( n = 10 each) : group I sham operation (group S) , group II BCP, group Ⅲ PBS and group IV minocyline (group M) . In group BCP, PBS and M, bone cancer pain was produced by injection of NCTC2472 fibrosarcoma cell suspension (2 x 105 cells) 10 μl into medullary cavity of calcaneus bone, while in group S, PBS solution 10 μl was injected instead of cancer cell suspension. In group PBS and M, PBS 5 μl and minocyline 5 μl (dissolved to 0.2 mmol/L in PBS)_were given IT immediately before cancer cell inoculation once a day for 11 consecutive days respectively. Mechanical pain threshold was measured at 1 d before cancer cell inoculation, and at 0, 3, 5, 7, 9 and 11d after cancer cell inoculation. Cold pain threshold was measured at 3, 7, 9 and 11d after cancer cell inoculation. The animals were killed after measurement of pain threshold and L4-6, segment of spinal cord was removed for determination of GFAP and CD11b expression by Western blot. Results Compared with group S, mechanical pain threshold was significantly increased at 3-11 d after cancer cell inoculation in group BCP and PBS, and at 3 and S d after cancer cell inoculation in group M, and cold pain threshold was significantly increased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was up-regulated in group BCP, PBS and M ( P < 0.05) . Compared with group BCP, mechanical pain threshold was significantly decreased at 3-11 d after cancer cell inoculation, cold pain threshold was significantly decreased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was down-regulated in group M ( P <0.05) . ConclusionThe activiton of gliocyte in the spinal cord is involved in the development of bone cancer pian in mice.     

脊髓胶质细胞在小鼠骨癌痛形成中的作用

Objective To evaluate the role of gliocyte in the spinal cord in the development of bone cancer pain (BCP) in mice. Methods Forty male C3H/He mice aged 8-10 weeks weighing 18-22 g were randomly divided into 4 groups ( n = 10 each) : group I sham operation (group S) , group II BCP, group Ⅲ PBS and group IV minocyline (group M) . In group BCP, PBS and M, bone cancer pain was produced by injection of NCTC2472 fibrosarcoma cell suspension (2 x 105 cells) 10 μl into medullary cavity of calcaneus bone, while in group S, PBS solution 10 μl was injected instead of cancer cell suspension. In group PBS and M, PBS 5 μl and minocyline 5 μl (dissolved to 0.2 mmol/L in PBS)_were given IT immediately before cancer cell inoculation once a day for 11 consecutive days respectively. Mechanical pain threshold was measured at 1 d before cancer cell inoculation, and at 0, 3, 5, 7, 9 and 11d after cancer cell inoculation. Cold pain threshold was measured at 3, 7, 9 and 11d after cancer cell inoculation. The animals were killed after measurement of pain threshold and L4-6, segment of spinal cord was removed for determination of GFAP and CD11b expression by Western blot. Results Compared with group S, mechanical pain threshold was significantly increased at 3-11 d after cancer cell inoculation in group BCP and PBS, and at 3 and S d after cancer cell inoculation in group M, and cold pain threshold was significantly increased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was up-regulated in group BCP, PBS and M ( P < 0.05) . Compared with group BCP, mechanical pain threshold was significantly decreased at 3-11 d after cancer cell inoculation, cold pain threshold was significantly decreased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was down-regulated in group M ( P <0.05) . ConclusionThe activiton of gliocyte in the spinal cord is involved in the development of bone cancer pian in mice.     

脊髓胶质细胞在小鼠骨癌痛形成中的作用

目的 评价脊髓胶质细胞在小鼠骨癌痛形成中的作用.方法 健康雄性C3H/He小鼠40只,周龄8～10周,体重18～22 g,随机分为4组(n=10):假手术组(S组)、骨癌痛组(B组)、PBS组(P组)和米诺环素组(M组).S组跟骨骨髓腔内注射PBS 10 μl;余3组跟骨骨髓腔内注射含2×105个骨纤维肉瘤细胞的PBS 10 μl制备骨癌痛模型,于造模前即刻开始PBS组鞘内注射PBS 5μl,M组鞘内注射米诺环素(用PBS溶解为0.2 mmol/L)5μl,1次/d,连续11 d.于造模前1 d、造模后即刻、3、5、7、9、11 d时测定机械痛阈;于造模后3、7、9、11 d机械痛阈测定结束后测定冷痛阈.痛阈测定结束后处死小鼠,取脊髓组织,测定神经胶质纤维酸性蛋白(GFAP)和CD11b的表达水平.结果 与S组比较,B组和P组造模后3-11 d时、M组造模后3、5 d时机械痛阈升高,B组、P组和M组造模后7～11 d时冷痛阈升高,脊髓CD11b和GFAP表达上调(P<0.05).与B组比较,M组造模后3-11 d时机械痛阈降低,造模后7-11 d时冷痛阈降低,脊髓CD11b和GFAP表达下调(P<0.05).结论 脊髓胶质细胞(星形胶质细胞和小胶质细胞)的激活参与了小鼠骨癌痛的形成.     

脊髓胶质细胞在小鼠骨癌痛形成中的作用

Objective To evaluate the role of gliocyte in the spinal cord in the development of bone cancer pain (BCP) in mice. Methods Forty male C3H/He mice aged 8-10 weeks weighing 18-22 g were randomly divided into 4 groups ( n = 10 each) : group I sham operation (group S) , group II BCP, group Ⅲ PBS and group IV minocyline (group M) . In group BCP, PBS and M, bone cancer pain was produced by injection of NCTC2472 fibrosarcoma cell suspension (2 x 105 cells) 10 μl into medullary cavity of calcaneus bone, while in group S, PBS solution 10 μl was injected instead of cancer cell suspension. In group PBS and M, PBS 5 μl and minocyline 5 μl (dissolved to 0.2 mmol/L in PBS)_were given IT immediately before cancer cell inoculation once a day for 11 consecutive days respectively. Mechanical pain threshold was measured at 1 d before cancer cell inoculation, and at 0, 3, 5, 7, 9 and 11d after cancer cell inoculation. Cold pain threshold was measured at 3, 7, 9 and 11d after cancer cell inoculation. The animals were killed after measurement of pain threshold and L4-6, segment of spinal cord was removed for determination of GFAP and CD11b expression by Western blot. Results Compared with group S, mechanical pain threshold was significantly increased at 3-11 d after cancer cell inoculation in group BCP and PBS, and at 3 and S d after cancer cell inoculation in group M, and cold pain threshold was significantly increased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was up-regulated in group BCP, PBS and M ( P < 0.05) . Compared with group BCP, mechanical pain threshold was significantly decreased at 3-11 d after cancer cell inoculation, cold pain threshold was significantly decreased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was down-regulated in group M ( P <0.05) . ConclusionThe activiton of gliocyte in the spinal cord is involved in the development of bone cancer pian in mice.     

脊髓胶质细胞在小鼠骨癌痛形成中的作用

Objective To evaluate the role of gliocyte in the spinal cord in the development of bone cancer pain (BCP) in mice. Methods Forty male C3H/He mice aged 8-10 weeks weighing 18-22 g were randomly divided into 4 groups ( n = 10 each) : group I sham operation (group S) , group II BCP, group Ⅲ PBS and group IV minocyline (group M) . In group BCP, PBS and M, bone cancer pain was produced by injection of NCTC2472 fibrosarcoma cell suspension (2 x 105 cells) 10 μl into medullary cavity of calcaneus bone, while in group S, PBS solution 10 μl was injected instead of cancer cell suspension. In group PBS and M, PBS 5 μl and minocyline 5 μl (dissolved to 0.2 mmol/L in PBS)_were given IT immediately before cancer cell inoculation once a day for 11 consecutive days respectively. Mechanical pain threshold was measured at 1 d before cancer cell inoculation, and at 0, 3, 5, 7, 9 and 11d after cancer cell inoculation. Cold pain threshold was measured at 3, 7, 9 and 11d after cancer cell inoculation. The animals were killed after measurement of pain threshold and L4-6, segment of spinal cord was removed for determination of GFAP and CD11b expression by Western blot. Results Compared with group S, mechanical pain threshold was significantly increased at 3-11 d after cancer cell inoculation in group BCP and PBS, and at 3 and S d after cancer cell inoculation in group M, and cold pain threshold was significantly increased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was up-regulated in group BCP, PBS and M ( P < 0.05) . Compared with group BCP, mechanical pain threshold was significantly decreased at 3-11 d after cancer cell inoculation, cold pain threshold was significantly decreased at 7-11 d after cancer cell inoculation, and expression of CD11b and GFAP was down-regulated in group M ( P <0.05) . ConclusionThe activiton of gliocyte in the spinal cord is involved in the development of bone cancer pian in mice.