P16抑癌基因在人完全性葡萄胎和正常胎盘组织中的表达

目的研究P16抑癌基因与葡萄胎发生的关系。方法分别取完全性葡萄胎和正常早孕流产标本各30例,用SABC免疫组织化学染色方法,检测P16抑癌基因在两种组织中的表达,并采用图像分析技术,对正常早孕绒毛组和葡萄胎组P16抑癌基因的表达情况进行对比分析。结果与正常绒毛相比,P16抑癌基因在完全性葡萄胎组织中的表达部位和表达量有显著性差异。结论P16抑癌基因与人完全性葡萄胎发生密切相关。     

人完全性葡萄胎中c-myc的表达及意义

目的研究c-myc基因在人完全性葡萄胎中的表达及其意义。方法取人完全性葡萄胎30例,正常早孕流产标本10例,用SABC免疫组织化学染色方法,检测c-myc基因在两种组织中的表达情况,并采用图像分析技术,对正常早孕绒毛组和完全性葡萄胎组c-myc的表达情况进行对比分析。结果与正常绒毛相比,c-myc基因在完全性葡萄胎组织中的表达量和表达的空间特异性有明显不同。结论 c-myc基因可能与完全性葡萄胎的发生密切相关。     

印记基因PEG10 在葡萄胎组织中的表达以及意义

目的:通过免疫组化方法,探讨印记基因PEG10在葡萄胎组织中的表达及其在早期鉴别葡萄胎妊娠中的应用价值。方法:选取经病理组织学诊断为完全性葡萄胎、部分性葡萄胎、正常早孕、难免流产的标本共计156例,采用免疫组织化学技术检测PEG10在其中的表达,研究遗传印记基因PEG10在葡萄胎妊娠以及非葡萄胎妊娠中的表达。结果:PEG10在四组蜕膜组织中均有表达,在难免流产组呈弱阳性表达,在正常早孕组呈弱阳性和中度阳性表达,在部分性葡萄胎组中呈中度阳性和强阳性表达,在完全性葡萄胎组中呈强阳性表达。PEG10在葡萄胎妊娠组表达明显增多于非葡萄胎妊娠组,两组比较具有显著性差异(P0.01),部分性葡萄胎组表达增多于难免流产组,两组比较差异有显著性(P0.05)。结论:遗传印记基因PEG10在葡萄胎组织中的表达明显高于正常早期妊娠和难免流产组,PEG10基因表达上调与葡萄胎的发生可能有重要关系,是否可将其用于病理诊断鉴别困难时的辅助手段。     

葡萄胎中MBD2表达及其相关基因甲基化芯片研究

用Real-time RT-PCR、Western blot和免疫组织化学方法分别检测了去甲基化酶MBD2(methyl-CpG-binding domain 2,MBD2)在完全型葡萄胎(complete hydatidiform mole,CHM)和正常早期妊娠绒毛中的表达,用甲基化DNA免疫沉淀MeDIP(methylated DNA immunoprecipitation)-甲基化芯片分析完全型葡萄胎和正常早期妊娠绒毛中相关基因的甲基化情况,用生物信息学分析筛选了差异甲基化基因并进行功能分类。MBD2的mRNA在完全型葡萄胎中的表达明显高于正常早期妊娠绒毛(P=0.0083),Western blot(P=0.0005)和免疫组织化学(P=0.0091)检测到MBD2蛋白表达与Real-time RT-PCR结果一致。结果显示MBD2在完全型葡萄胎中的表达显著高于正常早期妊娠绒毛组织(P<0.01),与正常早期妊娠绒毛组织相比较,完全型葡萄胎组织中相对有89个基因发生了去甲基化,其中85个基因可被映射到基因组图谱中,MBD2在完全型葡萄胎中的高表达及部分基因的去甲基化可能在完全型葡萄胎的发生中扮演了重...     

P57,P53,bcl-2,ki-67联合应用在葡萄胎诊断中的意义

目的:研究p57,P53,bcl-2,ki-67蛋白表达在完全性葡萄胎(CM)、部分性葡萄胎(PM)及水肿流产胎(HA)的诊断及鉴别诊断意义.方法:对21例完全性葡萄胎,28例部分性葡萄胎,18例水肿流产胎的标本进行4种抗体免疫组化分析,同时选取10例正常胎盘组织作为对照.结果:在CM中,p57表达不明显,而P53,bcl-2,Ki-67表达增强;在PM,HA及对照组中p57呈现高表达,P53,bcl-2,Ki-67则表达较弱.这四种抗体的表达在完全性葡萄胎与部分性葡萄胎、水肿流产胎及对照组之间的差异具有显著性(P＜0.01),而部分性葡萄胎与水肿流产胎、水肿流产胎与对照组之间差异不显著(P＞0.05).结论:p57和Ki-67表达对CM,PM和HA的鉴别诊断有重要作用,而P53,bcl-2表达对判断预后及预测恶变风险有意义.     

p21和p27基因在眼睑皮脂腺腺癌中的表达及意义

目的探讨p21和p27基因在眼睑皮脂腺腺癌中的表达差异。方法收集武汉大学人民医院和武汉大学中南医院病理科2000-2008年手术切除及活检的眼睑皮脂腺腺癌(eyelid sebaceous gland grandular cancer,ESGGC)标本共20例,另取癌周围组织5例作对照。采用免疫组织化学方法观察各组组织内p21和p27基因的表达。并利用HPIAS-2000图像分析系统测定p21和p27基因在以上各组中表达的平均光密度和平均阳性面积率。对各组组织中p21和p27基因表达的阳性面积率作双变量相关分析。结果 1.p21和p27基因在眼睑皮脂腺腺癌组织中呈低表达;p21和p27基因在癌旁组织中呈高表达。经单因素方差分析,组间有显著性差异(P0.05?。经q检验,眼睑皮脂腺腺癌与癌旁组织之间,p21和p27基因表达的平均光密度及阳性面积率有显著性差异(P0.05?。2.p21和p27基因之间的表达呈显著正相关。结论1.p21和p27基因在眼睑皮脂腺腺癌组织中异常表达,对眼睑皮脂腺腺癌的发生和发展起了重要作用;2.p21和p27基因之间的表达呈显著正相关,它们在皮脂腺腺癌的发生和发展过程中可能起协同作用。     

CXCL10和MMP-13在妊娠滋养细胞疾病滋养细胞中的表达及其临床意义

目的检测妊娠滋养细胞疾病滋养细胞中CXCL10和MMP-13表达情况,探讨其在滋养细胞疾病浸润和转移中的作用。方法采用免疫组织化学Powervision法检测40例早孕绒毛,30例葡萄胎,18例葡萄胎恶变(随访发生恶变),35例滋养细胞肿瘤(28例绒癌,7例胎盘部位滋养细胞肿瘤)中CXCL10和MMP-13的表达。结果CXCL10和MMP-13在滋养细胞肿瘤中表达阳性率和免疫反应性强度最高;在葡萄胎恶变组中表达阳性率和免疫反应性强度较高,但是低于在滋养细胞肿瘤中的表达阳性率和免疫反应性强度;在葡萄胎组和早孕绒毛组中表达阳性率和免疫强度较低。CXCL10和MMP-13在滋养细胞肿瘤中的表达,年龄<40岁组中表达低于年龄>40岁组;在临床分期分组(Ⅰ、Ⅱ)中表达低于临床分期分组(Ⅲ、Ⅳ);在FIGO预后评分分组低危组中表达低于高危组。结论CXCL10和MMP-13在早孕绒毛组织中低表达,而在滋养细胞肿瘤中高表达,提示其可能参与滋养细胞疾病的浸润和转移过程,因此联合检测CXCL10和MMP-13的表达可能对葡萄胎恶变的早期诊断以及对滋养细胞肿瘤的预后评估提供依据。     

p16在HBsAg和HBx转基因小鼠肝脏肿瘤中的表达

目的:探讨p16基因在由乙型肝炎病毒基因整合引起的小鼠肝细胞癌发生发展中的表达变化规律。方法:以乙肝病毒表面抗原基因(HBsAg)及X基因(HBx)定位整合转基因小鼠及对照小鼠的肝脏组织为标本,利用North-ern印迹、Western印迹及免疫组织化学检测p16在乙肝病毒基因定位整合转基因小鼠肝脏正常组织与肿瘤组织中的差异表达。结果:p16主要在小鼠胚胎期的肝脏中表达,在新生小鼠和成年小鼠的肝脏组织中几乎检测不到其表达;在HBsAg转基因小鼠和HBx转基因小鼠的肝脏肿瘤中,p16的表达明显升高。结论:p16基因在HBsAg或HBx诱导的肝细胞癌发生过程中被重新激活,也许发挥重要的作用。     

EB病毒与子宫颈癌发病的关系

目的 分析EB病毒感染与子宫颈的关系及其对抑癌基因p53表达的影响,探讨EB病毒的致癌机制。方法 采用免疫组织化学S-P法,分别检测59例宫颈鳞癌,19例正常宫颈组织的EB病毒（Epstein-Barr virus,EBV）及抑癌基因p53蛋白的表达情况,并进一步分析宫颈癌组织EBV感染与抑癌基因p53表达的关系。结果 EBV阳性表达率在宫颈癌及正常宫颈组分别为64．4％和21．1％,2组间差异有显著性（P〈0．05）;p53在宫颈癌组织中的阳性表达率为64．4％,明显高于正常宫颈组26．3％,（P〈0．05）。EBV感染与非感染的宫颈癌组织中,p53的阳性表达率分别为78．9％与38．1％,2组间差异有显著性（P〉0．05）。结论 EBV病毒感染与宫颈癌的发病密切相关,但其机制可能是通过影响抑癌基因P53表达而致癌。     

p27和p53基因在大肠癌中的表达及临床意义

目的 研究大肠癌患者癌组织中p27、p53基因的表达及其相互之间的关系,以探讨p27、p53基因在大肠癌发生中的作用及临床意义。方法 运用原位杂交方法及免疫组化SP法检测58例大肠癌组织及正常黏膜中p27mRNA和P27蛋白的表达,同时运用免疫组化法分析相同组织中P53蛋白表达状况。结果 p27mRNA在大肠癌组织及正常黏膜中的表达阳性率均为100%。P27蛋白在大肠癌组织中的表达阳性率为55.17%,在正常黏膜中的表达阳性率为96.55%（P〈0.01）;癌组织中P53蛋白表达阳性率为53.45%,正常黏膜未见P53蛋白表达（P〈0.01）;大肠癌组织中P27与P53蛋白表达无明显相关性。P27蛋白的表达与肿瘤分化程度呈负相关（P〈0.01）,与临床其它病理因素均无相关性（P〉0.05）。大肠癌组织中P53蛋白表达与临床病理因素亦无相关性（P〉0.05）。结论 P27蛋白表达的调控主要在转录后水平,P27蛋白检测可作为评价大肠癌恶性程度和预后判断的重要指标。P27及P53蛋白在大肠癌的发生发展过程中具有重要作用。     

MiR‐30a‐5p inhibits proliferation and metastasis of hydatidiform mole by regulating B3GNT5 through ERK/AKT pathways

Hydatidiform moles are gestational trophoblastic disease. They are abnormal proliferations of trophoblast cells that have the potential to become cancerous. miR‐miR30a‐5p is a tumour suppressor that participates in the development of numerous diseases. However, the role of miR‐30a in hydatidiform moles and the mechanisms underlying its effects are presently unclear. This study explored the levels of miR‐30a and B3GNT5 expression in human hydatidiform mole tissue. The results showed that miR‐30a and B3GNT5 were differentially expressed in normal placenta and hydatidiform mole, and miR‐30a decreased cell proliferation, invasion and migration in trophoblast cell lines. Upon further examination, it was confirmed that miR‐30a directly targeted the 3’untranslated region of B3GNT5 using a dual‐luciferase assay. The results of the present study also revealed that miR‐30a reduced the proliferation, invasion and migration ability in JAR and BeWo cells by regulating B3GNT5, which may inactivate the ERK and AKT signalling pathways. This study demonstrated that miR‐30a was a novel target B3GNT5 that serves an important role in the development of hydatidiform moles, suggesting that miR‐30a may serve as a novel potential biomarker or useful diagnostic and therapeutic tool for hydatidiform moles in clinical settings.     

葡萄胎与细菌L型感染关系的探讨

本文应用革兰氏染色和免疫组化等技术对110例葡萄胎进行了研究。结果发现28.2％葡萄胎中能检出L型。26/31例免疫组化染色证明葡萄胎组织内亦有L型抗原存在。第1次清宫前有不规则性阴道流血者,其水肿绒毛或蜕膜组织中L型检出率明显高于无流血者,两者有显著性差异(P<0.005)。并讨论了宫腔L型感与葡萄胎发生的可能关系。     

Protein phosphatase 1A (PPM1A) is involved in human cytotrophoblast cell invasion and migration

Trophoblast invasion is crucial for embryo implantation and placentation. Excessive trophoblast invasion leads to hydatidiform moles and choriocarcinoma. PPM1A is a phosphatase which dephosphorylates and inactivates a broad range of substrates, including TGF-β, MAP kinases, p38 and JNK kinase cascades, and is involved in tumor suppression. The objective of this study was to investigate the expression of PPM1A in normal and malignant human placenta and its role in trophoblast invasion, which shares many similarities with invasion of tumor cells. By Western blotting and immunocytochemistry, significantly higher expression of PPM1A in human placental villi at term was found as compared with that during the first trimester. Furthermore, the expression level of PPM1A protein in hydatidiform moles was lower compared with that during normal pregnancy. We further investigated the function of PPM1A in extravillous trophoblast cell line HTR8/SVneo. Transwell migration and Matrigel invasion assays demonstrated that PPM1A siRNA significantly promoted the motility and invasiveness of the cells. Gelatin zymography showed that knockdown of PPM1A with siRNA elevated the expression of pro-matrix metalloproteinase pro-(MMP)-9, but down-regulated tissue inhibitors of metalloproteinases (TIMP)-2. The present data indicate that PPM1A plays a critical role in the regulation of normal placentation by inhibiting trophoblast migration and invasion.     

A familial case of recurrent hydatidiform molar pregnancies with biparental genomic contribution

Hydatidiform mole is a benign trophoblastic neoplasia characterized by an abnormal development of the embryo and proliferation of placental villi. Using microsatellite markers amplified by the polymerase chain reaction, we have performed a genetic study on eight independent molar tissues occurring in two sisters. Karyotype and genotype data demonstrate a diploid and biparental constitution in seven of the analyzed moles suggesting a common mechanism underlying the etiology of the various molar pregnancies in this family. The data reported here suggest that complete and partial hydatidiform moles are not always separate entities and that women with familial recurrent hydatidiform moles are homozygous for an autosomal recessive mutation. Electronic Publication     

Expression of Fas/Fas ligand by decidual leukocytes in hydatidiform mole

Complete hydatidiform moles are entirely paternally derived and, therefore, represent a complete intrauterine allograft that might be expected to provoke an altered maternal immune response compared with that of normal pregnancy. Uterine decidua contains a large leukocyte population, of which 10%-20% are T lymphocytes. Fas ligand (FasL) expression by placental trophoblast may induce apoptosis of Fas+ lymphocytes, thereby facilitating immune tolerance and survival of the molar trophoblast. Our previous studies have shown an increase in activated CD4+ decidual T cells in molar pregnancy compared with normal pregnancy. This study was designed to characterize and quantitate Fas/FasL expression by decidual leukocytes in complete and partial hydatidiform mole compared with that in normal early pregnancy using single and double immunohistochemical labeling (i.e., avidin-biotin-peroxidase and avidin-biotin-alkaline phosphatase). A significant increase was found in Fas and FasL expression by decidual CD4+ T cells in complete (Fas+, P = 0.0106; FasL+, P = 0.0081) and partial (Fas+, P = 0.0131; FasL+, P = 0.0051) hydatidiform moles, as was a significant decrease in Fas expression by decidual CD8+ T cells in complete (P = 0.0137) and partial (P = 0.0202) hydatidiform mole compared with normal early pregnancy. The implications of altered Fas/FasL status of decidual T-cell subsets in hydatidiform mole are also discussed.     

The hydatidiform mole

ABSTRACT

The hydatidiform mole (HM) is a placental pathology of androgenetic origin. Placental villi have an abnormal hyperproliferation event and hydropic degeneration. Three situations can be envisaged at its origin: 1. The destruction/expulsion of the female pronucleus at the time of fertilization by 1 or 2 spermatozoa with the former being followed by an endoreplication of the male pronucleus leading to a complete hydatidiform mole (CHM) 2. A triploid zygote (fertilization by 2 spermatozoa) leading to a partial hydatidiform mole (PHM) but can also lead to haploid and diploid clones. The diploid clone may produce a normal fetus while the haploid clone after endoreplication generates a CHM 3. A nutritional defect during the differentiation of the oocytes or the deterioration of the limited oxygen pressure during the first trimester of gestation may lead to the formation of a HM.

In countries with poor medical health care system, moles (mainly the CHM) can become invasive or, in rare cases, lead to gestational choriocarcinomas.     

Expression of renin and angiotensinogen genes in the human placental tissues

The expression of renin and angiotensinogen genes in the human placenta and related tissues has been examined by RNA blot hybridization analysis with specific human complementary DNA (cDNA) probes. Renin mRNA was detectable in the chorion throughout pregnancy and in the hydatidiform moles, but not in the decidua, amnion or myometrium. The relative concentration of renin mRNA in the chorion was at the highest level in early pregnancy and decreased thereafter, while the total amount contained in the whole placenta was at the lowest level in early pregnancy, and increased thereafter, reaching at term about one-sixth of the total renin mRNA in the kidney. Hydatidiform moles had an even higher concentration of renin mRNA than the early chorion. There was no significant difference in either the relative concentration or the total renin mRNA content in the placentae from 4 normal and 4 toxemic pregnancies. Angiotensinogen mRNA was undetectable in any of the placental tissues, hydatidiform moles or myometrium. These results show that renin is synthesized in the placenta, possibly to play some physiological role locally by utilizing angiotensinogen which is abundantly present in the maternal systemic circulation.