食管鳞癌组织中的神经纤维分布

目的:探讨食管鳞癌组织中神经纤维的分布情况.方法:应用免疫组化ABC法,探查手术切除的食管鳞癌组织里S100及GAP-43阳性神经纤维的分布情况,并分析其与患者临床病理参数的关系.结果:相对于正常组织,食管鳞癌组织中存在相当数量的S100及GAP-43阳性神经纤维(束)不规则地分布于肿瘤细胞之间,且S100阳性纤维密度大于GAP-43阳性纤维密度;统计分析显示肿瘤组织中纤维密度与患者的肿瘤大小、淋巴结转移相关.结论:食管鳞癌组织中确实存在神经纤维分布,并对肿瘤发展起一定作用.     

食管鳞癌VEGF-C mRNA和CD31表达及其意义

研究食管鳞癌血管内皮生长因子C(VEGF-C)mRNA和CD 31的表达,探讨VEGF-C促食管鳞癌淋巴转移的作用。应用原位杂交法检测43例食管鳞癌组织VEGF-C mRNA表达,CD 31免疫组织化学染色标记血管、淋巴管内皮细胞,并计数肿瘤组织的微血管密度(MVD)。结果显示,食管鳞癌组织VEGF-C mRNA阳性19例(41.86%),MVD平均为76.36±20.30/mm~2。VEGF-C mRNA表达与食管鳞癌淋巴结转移、TNM分期和肿瘤浸润深度相关(p<0.05或p<0.01);而与肿瘤组织学分级无关(p>0.05)。MVD与食管鳞癌淋巴结转移、TNM分期的相关性有统计学意义(p<0.05);而与肿瘤浸润深度和组织学分级的相关性则无统计学意义(p>0.05)。VEGF-C mRNA表达阳性者MVD高于表达阴性者,两者比较具有显著性差异(p<0.05)。研究提示VEGF-C促进了肿瘤诱导的淋巴管新生和血管新生,在食管鳞癌的淋巴转移中起重要作用。     

食管鳞状细胞癌中MMP-9、CD-147的表达及意义

目的：探讨基质金属蛋白酶9（MMP-9）和CD-147在食管鳞状细胞癌的表达及其与肿瘤浸润转移的关系。方法：应用免疫组化S-P法观察57例食管鳞癌组织中MMP-9、CD-147的表达,并探讨其与食管鳞癌临床病理资料的关系。结果：MMP-9、CD-147在癌组织中的阳性表达率分别为82．46％,64．91％;在癌旁组织中的阳性表达率分别是29．82％,8．77％。在食管鳞癌中,MMP-9及CD-147的表达均与食管鳞癌的浸润深度有关,与分化程度无明显关联;有淋巴结转移的病例阳性表达率明显高于无淋巴结转移组。结论：MMP-9及CD-147的表达均与食管鳞癌的浸润深度及淋巴结转移有关。     

食管鳞癌组织中TNFAIP3的表达及其预后意义

目的研究肿瘤坏死因子α诱导蛋白3(tumor necrosis factorα-induced protein 3, TNFAIP3)在食管鳞癌中表达的临床病理意义及其对鳞癌预后的判断价值。方法免疫组织化学法检测100例随访食管鳞癌及80例癌旁组织中TNFAIP3蛋白的表达,并分析了其与食管鳞癌临床病理特征及预后的关系。结果 TNFAIP3在食管鳞癌中高表达阳性率为47.0%(47/100),显著高于癌旁组织中的高表达率15.0%(12/80),且与肿瘤的分化程度有关;生存分析显示高表达TNFAIP3的患者预后不良,单因素生存分析显示TNFAIP3的表达、肿瘤的浸润深度、淋巴结转移、临床分期与食管鳞癌预后密切相关,多因素生存分析显示TNFAIP3的表达、肿瘤的浸润深度、淋巴结转移、临床分期为食管鳞癌的独立预后预测因子。结论表达增高的TNFAIP3可能参与了食管鳞癌的发生发展,TNFAIP3的高表达可能成为食管鳞癌的独立预后因子。     

MTA1蛋白在食管鳞癌中的表达和临床意义

目的:探讨肿瘤转移相关基因1(MTA1)蛋白表达与食管鳞癌临床病理参数之间的关系.方法:应用免疫组化SP法和Western blotting方法检测50例食管鳞癌组织中MTA1蛋白的表达.结果:50例食管鳞癌组织中42例MTA1蛋白阳性表达,阳性率为84%.而癌旁组织中10例MTA1蛋白阳性表达,阳性率为20%,差异有显著性(P＜0.05);MTA1高表达与组织分化程度和淋巴结转移有关(P＜0.05),与年龄、性别、肿瘤大小无关(P＞0.05).结论:MTA1在食管鳞癌中高表达,与食管鳞癌的疾病进展密切相关,并有望成为基因治疗的新靶点.     

食管鳞状细胞癌中HDGF、VEGF表达与微血管形成的关系

目的:研究食管鳞状细胞癌中肝癌衍生生长因子(HDGF)、血管内皮生长因子(VEGF)的表达及其与微血管形成的关系。方法:通过免疫组化SABC法检测和比较68例食管鳞癌、20例切缘正常组织中HDGF、VEGF的表达和CD34标记的微血管密度(MVD),分析HDGF和VEGF表达之间的关系及其与食管鳞癌患者临床病理因素和食管癌组织MVD值的关系。结果:食管鳞癌组织中HDGF(63.2%)和VEGF(72.1%)的阳性表达率均明显高于切缘正常粘膜组织(15.0%、20.0%)(P0.05),食管鳞癌组织和切缘正常粘膜组织中的MVD值分别为35.48±5.75和13.50±2.1(P0.05)。食管鳞癌组织HDGF的阳性表达率仅与其临床分期明显相关(P0.05),而VEGF的阳性表达率与其淋巴结转移、临床分期均显著相关(P0.05),二者在食管鳞癌组织中的表达呈显著正相关(P0.05)。食管鳞癌组织中HDGF、VEGF阳性表达组MVD值均明显高于HDGF、VEGF阴性表达组(P0.05)。结论:HDGF可能通过诱导VEGF的产生,从而促进血管生成,参与食管鳞癌的发生、发展及转移。     

MRP2 蛋白在食管鳞癌中的表达及其与化疗耐药的相关性

目的:探讨MRP2蛋白在食管鳞癌组织中的表达及其与食管癌化疗耐药的关系。方法:收集原发性食管鳞癌手术标本70例,采用免疫组织化学Envision法检测食管鳞癌组织及其癌旁组织中MRP2蛋白的表达情况,并采用MTT法检测食管鳞癌组织对临床常用化疗药物的敏感性,分析其表达与食管癌化疗耐药的关系。结果:70例食管鳞癌组织及其癌旁正常组织中的阳性表达率分别为58.6%及5.0%。MRP2蛋白在食管鳞癌组织中的阳性表达率明显高于癌旁正常食管组织(P<0.01)。食管鳞癌组织对环磷酰胺、5-氟尿嘧啶、吉西他滨、顺铂、卡铂、阿霉素、长春瑞滨、羟喜树碱等化疗药物的敏感性与其相应癌组织中MRP2表达明显相关(P<0.01)。结论:MRP2的表达与食管鳞癌对多种化疗药物耐药有较好的相关性,推测食管鳞癌组织中MRP2的高表达可能对化疗耐药性的发生发展具有促进作用。     

NFE2L1在食管鳞癌中的表达及临床意义

目的:通过检测食管鳞癌标本中核因子E2相关因子1(NFE2L1)的表达情况,探究NFE2L1在食管鳞癌发生发展中的作用,为食管鳞癌的诊治以及预后评估提供新的思路。方法:收集我校附院2016-2017年经病理组织学检查诊断为食管鳞癌的手术标本40例及其对应的癌旁组织并从NCBI数据库下载GEO测序数据,应用定量PCR、免疫组化和生物信息分析等方法检测分析NFE2L1基因的表达情况。结果:在食管鳞癌组织中,NFE2L1表达阳性31例(77.5%),癌旁组织阳性表达17例(42.5%),两组比较差异显著有统计学意义(P0.001);进一步发现NFE2L1的阳性表达与肿瘤分化程度和淋巴转移相关(P0.05)。但在不同年龄、性别、浸润深度及不同部位之间差异无统计学意义。GEO数据分析结果显示NFE2L1在食管鳞癌组织显著高表达(P0.01),只是未达到显著差异表达的阈值标准(即变化倍数小于2倍)。结论:NFE2L1在食管鳞癌中高表达,表达的高低与食管鳞癌的发生进展密切相关。     

猫视神经中S100蛋白表达的年龄相关变化

比较老年猫和青年猫视神经S100蛋白表达及胶质细胞的年龄相关变化,探讨其可能的生理作用.取老年猫(10～13龄)和青年猫(1～3龄)各4只的颅内视神经相应部分作组织切片,用免疫组织化学ABC法标记S100免疫阳性(S100～IR)细胞,Marsland-Gless染色显示胶质细胞.光镜下采用图像分析系统计数视神经中S100-IR细胞密度、胶质细胞密度及阳性反应灰度值.视神经中棕黄色S100-IR细胞分布均匀,Marsland-Gless染色的纤维横断面及胶质细胞均呈棕红色.与青年猫相比,老年猫视神经中胶质细胞密度明显增大;S100-IR细胞密度显著增加(P<0.01),胞体较大,阳性较强(灰度值显著减小,P<0.01);S100-IR细胞在胶质细胞中所占比例亦显著增大.结果表明S100-IR细胞呈明显的年龄相关性增生,这可能对衰老的神经纤维起保护作用.     

Skp2和P27在食管鳞状细胞癌中表达及其临床意义

目的:研究S期激酶相关蛋白2(Skp2)与细胞周期素抑制因子P27在人食管鳞状细胞癌中蛋白冰平的表达差异,分析二基因的相互关系及其与食管鳞癌浸润深度、组织学分级、淋巴结转移等临床病理因素间的关系,探讨Skp2和P27在食管鳞癌发生发展过程中的作用及其临床意义.方法:应用免疫组化检测49例食管鳞癌及其切缘正常组织中Skp2和P27的表达,用PearsonX<'2>检验分析二者的表达在两组间是否有差别;用Pearson X<'2>检验和Fisher's确切概率法分析Skp2和P27表达与食管鳞癌患者性别、年龄、临床分期、病理组织学分级、淋巴结转移等临床病理因素间的关系;用Pearson相关系数分析食管鳞癌中Skp2和P27两者表达的相关性;结果:Skp2在食管鳞癌及其切缘正常粘膜组织中的阳性表达率分别为57.1%和20.0%,(P<0.05).P27在食管鳞癌及其切缘正常粘膜组织中的阳性表达率分别为51.0%和85.0%,(P<0.05).Skp2和P27的表达与临床分期、组织学分级、淋巴结转移显著相关,与患者性别、年龄无显著相关,且二者在食管鳞癌中表达呈显著负相关.结论:食管鳞癌中Skp2基因在蛋白水平高表达,在切缘正常粘膜组织中低表达,P27蛋白表达与Skp2蛋白表达之间呈负相关.Skp2和P27表达与食管鳞癌肿瘤临床分期、组织学分级、淋巴结转移等临床病理因素密切相关.     

Immunohistochemical observation of growth-associated protein 43 (GAP-43) in the developing circumvallate papilla of the rat

The distribution and development of growth-associated protein 43 (GAP-43)-like immunoreactivity (-LI) in the rat circumvallate papilla (CVP) were compared to those of protein gene product 9.5 (PGP 9.5)-LI. In the adult, thick GAP-43-like immunoreactive (-IR) structures gathered densely in the subgemmal region. Some of these further penetrated the apical epithelium and trench wall epithelium. At least two types of GAP-43-IR structures were recognized; taste bud-related and non-gustatory GAP-43-IR neural elements. Immunoelectron microscopy revealed that GAP-43-LI was localized predominantly in the Schwann cells, and a few axons displayed GAP-43-LI in the lamina propria. In the trench epithelium, GAP-43-LI was detected in the cytoplasmic side of the axonal membrane. Some intragemmal GAP-43-IR axons made synaptic-like contacts with taste bud cells. At least four developmental stages were defined on the basis of the changes in distribution of GAP-43-LI. In stage I [embryonic day (E) 16–17] GAP-43-IR structures accumulated at the lamina propria just beneath the newly-formed circumvallate papilla. In stage II (E18–19) GAP-43-IR nerve fibers began to penetrate the apical epithelium. In stage III [E20-postnatal day (P) 0] GAP-43-IR nerve fibers first appeared in the trench wall epithelium. Penetration of GAP-IR nerve fibers occurred in the inner trench wall epithelium first, and then in the outer trench wall epithelium. In stage IV (P1-) the distribution of GAP-43-LI was similar to that observed in the adult; but the density of GAP-43-LI was much higher than in adults. PGP 9.5-LI showed a similar distribution pattern to that of GAP-43-LI, except for round-shaped cells in the apical epithelium at the late embryonic stages, and in taste bud cells and intralingual ganglionic cells which lacked GAP-43-LI. The similarities in distribution patterns of GAP-43-LI and PGP 9.5-LI during the development and mature circumvallate papilla suggest that GAP-43 may be a key neuronal molecule for induction and maintenance of the taste buds.     

Quantitative comparison of growth-associated protein GAP-43, neuron-specific enolase, and protein gene product 9.5 as neuronal markers in mature human intestine.

This study was performed to compare GAP-43, PGP 9.5, synaptophysin, and NSE as neuronal markers in the human intestine. GAP-43-immunoreactive nerve fibers were abundant in all layers of the ileum and colon. GAP-43 partially co-localized partially with every neuropeptide (VIP, substance P, galanin, enkephalin) studied. All neuropeptide-immunoreactive fibers also showed GAP-43 reactivity. By blind visual estimation, the numbers of GAP-43-immunoreactive fibers in the lamina propria were greater than those of PGP 9.5, synaptophysin, or NSE. In the muscle layer, visual estimation indicated that the density of GAP-43-immunoreactive fiber profiles was slightly greater than that of the others. The number and intensity of GAP-43-, PGP 9.5-, and NSE-immunoreactive fibers were estimated in sections of normal human colon and ileum using computerized morphometry. In the colon, the numbers of GAP-43-immunoreactive nerve profiles per unit area and their size and intensity were significantly greater than the values for PGP and NSE. A similar trend was observed in the ileum. Neuronal somata lacked or showed only weak GAP-43 immunoreactivity, variable PGP 9.5 immunoreactivity, no synaptophysin immunoreactivity, and moderate to strong NSE immunoreactivity. We conclude that GAP-43 is the superior marker of nerve fibers in the human intestine, whereas NSE is the marker of choice for neuronal somata. (J Histochem Cytochem 47:1405-1415, 1999)     

Transitional expression of OX-2 and GAP-43 glycoproteins in developing rat cochlear nerve fibers

The OX-2 and GAP-43 glycoproteins are two proteins involved in neuronal cell-to-cell interaction and/or growing of dendrites and axons. Therefore, for the auditory receptor the expression of these proteins could provide information on the afferent and efferent nerve fiber organization. The expression and distribution of OX-2 and GAP-43 were analyzed during the auditory receptor development and maturation (from embryonic day E13 to postnatal day P22). Both glycoproteins were early recognized in the cochleae of E13 rats. Then, they slowly but progressively disappeared, being absent when the animals reached the P22 postnatal day. At E13, a weak OX-2 expression was restricted to the perikaryon of the spiral ganglion neurons, while in the same period a strong GAP-43 immunostaining was found in both the neuronal perikaryon and the neurites. During the rat embryonic period (E13 to birth) the expression of both glycoproteins appeared progressively restricted to the neurites. During the rat postnatal period (P0 to P22), OX-2 and GAP-43 exhibited a dissimilar distribution pattern. The OX-2 glycoprotein appeared in the afferent, efferent and fibers of the auditory nerve, while the GAP-43 glycoprotein only appeared in the efferent nerve fibers. Present data suggest that OX-2 and GAP-43 could act as two complementary glycoproteins during the development, organization, and maturation of the cochlear nerve fibers. While both glycoproteins could participate in axonal growing and orientation, OX-2 could also be involved in a similar process for auditory dendrites.     

Immunocytochemical evidence of plasticity in the nervous structures of the rat lower lip

In this immunocytochemical study we investigated the distribution of nervous structures in the lower lip of adult rats. The region is characterized by a rich cutaneous and mucosal sensory innervation originating from terminal branches of the trigeminal system. Lower lip innervation was investigated by detection of the general neuronal marker protein gene product 9.5 (PGP 9.5) and the growth-associated protein 43 (GAP-43), a neurochemical marker of neuronal plasticity. The entire neural network of both cutaneous and mucosal aspects was stained by the antibody to PGP 9.5. In particular, nerve fibers were observed in the submucosal and the subepithelial plexuses. Thin immunoreactive fibers were observed within the epithelial layers ending as free fibers or as fibers associated with immunopositive Merkel cells. Well-identified anatomical structures receiving sensory or autonomic innervation were also surrounded by PGP 9.5-ir nerve fibers, in particular, hair follicles, vibrissae, glands, and blood vessels. GAP-43-immunostained nerve fibers were observed in all these structures; however, they were generally less numerous than the PGP 9.5-immunoreactive elements. An equal amount of PGP 9.5 and GAP-43 immunoreactivity occurred, in contrast, in the subepidermal and the submucosal plexuses, or in the epidermis and the mucosal epithelium. The present results show that GAP-43 is normally expressed in the mature trigeminal sensory system of the rat. Skin and oral mucosa are characterized by continuous remodeling that may also involve the sensory nervous apparatus. Continuous neural remodeling, regeneration and sprouting may be the reason for the observed expression of GAP-43.     

Development of the innervation of long bones: expression of the growth-associated protein 43

It has been known from clinical and experimental observations that the peripheral nervous system is involved in the development of long bones. Expression of growth-associated protein 43 (GAP-43/B-50) was found in axonal growth cones during embryonic and postnatal ontogeny as well as in regenerating axons after nerve injury. The aim of the present study was to examine the occurrence of growing nerve fibers in rat tibia from gestational day 16 (GD 16) to postnatal day 28 (PD28). An indirect immunoenzymatic reaction using antibodies raised against GAP-43 was applied to detect outgrowing nerve fibers penetrating into the developing bone. On GD 16 and GD 17 no GAP-43-immunoreactive (IR) fibers were observed in the close vicinity of bone rudiments. On GD19 GAP-43-IR fibers were scarcely present within the periosteum of the central portion of the diaphysis. In the perichondrium surrounding the proximal epiphysis, nerve fibers were first detected around birth. From PD1 onward, numerous fibers were seen in the fibrous buds of the perichondrium at the epi-metaphyseal junction (Ranvier's grooves), some of them being adjacent to the blood vessels. Nerve fibers penetrating into the bone and located in the bone marrow, predominantly associated with blood vessels, were first observed on GD21 and their number increased with further development. They were initially located in the central portion of the diaphysis and later extended towards the metaphyses. On PD4 an increased number of GAP-43-IR fibers appeared in the perichondrium of proximal and distal epiphyses. In the fibrous strands penetrating into the epiphyses and in the secondary ossification centers, nerve fibers were first observed on PD10. From PD14 onward the pattern of tibial innervation remained unchanged but the intensity of GAP-43 immunostaining visibly decreased. The present study demonstrates that developing long bones of rat hindlimbs are supplied by growing nerve fibers immunoreactive for GAP-43 from GD 19 onward. Time and location of their appearance were at least partially correlated with known events taking place during long bone development, e.g. formation of primary and secondary ossification centers. Decreased expression of GAP-43 immunoreactivity in later developmental stages is believed to reflect nerve fiber maturation.     

氢氧化钠瘤内注射通过抗血管生成作用抑制肝癌生长的机制研究

目的：研究氢氧化钠溶液瘤内注射对肝癌的生长抑制作用并探索其机制。方法：对SMMU-LTNM肝癌裸鼠皮下模型进行2%浓度的氢氧化钠溶液瘤内注射,检测肿瘤组织微血管密度、HIF-1α和VEGF的表达情况。结果：与生理盐水瘤内注射组相比,氢氧化钠显著抑制肿瘤生长（P〈0.01）、降低肿瘤微血管密度（P=0.01）、抑制肿瘤组织HIF-1α和VEGF的表达（P=0.02和P=0.01）。结论：氢氧化钠瘤内注射可有效抑制肝癌生长,主要机制可能是抗血管生成作用。     

脑肿瘤及脑肿瘤图像分类的研究进展

脑肿瘤分类的方法很多,目前尚无统一的分类方法,并且各种肿瘤的组织发生与病理特征不同,其良性与恶性以及物学特性也不一样。通常按组织学可分类如下：（1）发源于神经胶质的肿瘤：星形细胞瘤、少支胶质细胞瘤、髓母细胞瘤等。（2）发源于脑膜的肿瘤：脑膜瘤、脑膜肉瘤、蛛网膜囊肿等。（3）发源于垂体的肿瘤：厌色细胞腺瘤,嗜酸、嗜碱性细胞腺瘤。（4）发源于颅神经的肿瘤：听神经瘤、三又神经瘤等各种神经鞘瘤。（5）发源于胚胎残余组织：颅咽管瘤、脊索瘤、皮样囊肿等。（6）发源于血管细胞：血管瘤及血管网织细胞瘤等。（7）由其它部位转移或侵入的肿瘤：各种转移瘤及鼻咽癌等。     

鱼类动眼神经的形态学研究

目的：应用生物胞素法观察罗非鱼动眼神经的形态分布。方法：本实验用罗非鱼,10只（性别不限）,体长12．16cm,动物浸入140mg／L三卡因间氨苯酸乙脂甲磺酸盐{tricainemethanesulfonate（MS222）}溶液中麻醉,在手术显微镜下暴露动眼神经,通过生物胞素（Biocytin）结晶追踪技术研究定位硬骨鱼类动眼神经的形态分布。结果：①被标记的神经纤维长而粗细不等,排列比较松散,从后外向前内方向行走,逐渐靠近,终于位于中脑腹侧部的动眼神经核细胞,同时可以观察到有些神经纤维交叉到对侧。②神经核细胞呈圆形和卵圆形,大小不一,亦可见神经元的突起,有的突起呈螺旋状连于胞体,有的呈线状连于胞体,形成神经终末及突触联系,并可见到多极神经元,并在神经纤维之中也可以见到少数神经核细胞,但部分标记结构并不太完整,有些标记的神经细胞和神经纤维不是很清楚。结论：鱼类动眼神经纤维在中脑内的走行与其他动物基本一致,动眼神经核位于中脑水管腹侧部。     

原发性肝癌染色体8p、16q遗传变异的研究

目的：分析人肝癌（HCC）组织中染色体8p、16q部分基因及染色体片段的遗传变异及与临床病理关系,初步筛选HCC相关的抑癌基因。方法：应用聚合酶链反应-变性聚丙烯酰胺凝胶-银染法分析45例HCC组织标本中染色体8p和16q的杂合性丢失（LOH）及微卫星不稳定性（MSI）。结果：发生LOH的总频率为68.89%（31/45）,其中D16S511位点的发生LOH率最高为53.33%（24/45）,其次是D8S261（39.02%,16/41）和D8S499（34.88%,15/43）。MSI出现的总频率为11.11%（5/45）,出现在三个微卫星位点（D8S261、D8S499及D16S511）上。结论：染色体16q23、8p22-21.3及8p12区域的LOH发生频率高,其可能存在与HCC发生发展相关的新的抑癌基因,特定位点的遗传变异可能与HBV感染、临床病理恶性程度等预后因素相关。