STUDY OF LOSS OF HETEROZYGOSITY AT DCC AND APC/MCC GENETIC LOCI OF GASTRIC CANCER

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胃癌组织中抑癌基因APC／MCC杂合性缺失的研究

应用多聚酶链反应（ＰＣＲ）与限制性片段长度多态性分析法（ＲＦＬＰ），对４５例手术切除胃癌组织腺癌性息肉基因（ＡＰＣ）／结直肠癌突变基因（ＭＣＣ）杂合性缺失（ＬＯＨ）进行分析。结果表明ＡＰＣ、ＭＣＣ基因ＬＯＨ串分别为２１．７％（５／２３）和３１．３％（５／１６）．ＡＰＣ／ＭＣＣ缺失率为３０．０％（９／３０）。ＬＯＨ率在肠型及胃型胃癌中无明显差异，与肿瘤大小、组织学分类、浸润深度、淋巴转移及临床分期无关。一例早期胃癌出现ＭＣＣ基因缺失。结果提示ＡＰＣ／ＭＣＣ基因ＬＯＨ与两型胃癌的早期发生及发展有关。

食管癌APC/MCC基因杂合缺失的研究

目的 研究APC/MCC基因杂合性缺失 (LOH)与食管癌发生发展的关系。方法 应用多聚酶链反应技术及限制性片段长度多态现象对 46例食管癌APC和MCC基因的LOH进行了分析。结果 食管癌APC和MCC基因LOH阳性表达分别为 2 9.0 % (9/31)和 33 .3 % (8/2 4)。结论 APC、MCC基因的LOH是食管癌的常见改变 ,可能参与了食管癌的发生。

大肠癌组织APC/MCC和DCC基因杂合缺失的研究

采用聚合酶链反应(PCR)技术.并配合限制性片段长度多态性(RFLP)分析。对41例大肠癌组织APC/MCC和DCC基因的杂合缺失(LOH)进行研究。APC基因LOH率为28.0％(7/25),MCC基因LOH率为36.40％(8/22),两者综合分析LOH率为38.9％(14/38)。DCC基因LOH率为55.3％(21/38)。DCC基因在有淋巴结转移组的LOH率(80.0％),显著高于无淋巴结转移组(39.1％)(P<0.05),在Dukes C、D期组的LOH率(71.4％)显著高于A、B期组(35.3％)。以上结果提示,APC/MCC和DCC基因的LOH是大肠癌常见的基因改变,DCC基因LOH的测定有可能成为大肠癌病人预后评估的指标。

Abnormal Change of p53 Gene in Gastric and PrecancerousLesions and APC Gene Deletion in Gastric Carcinoma and Near Tissues

p53 gene mutation (exon4, 5, 6, 7, 8 and intron6) in gastric cancer and precancerous lesions and p53 gene (exon4 and ontron6), APC gene deletion in gastric carcinomas were studied by PCR/SSCP and PCR/RFLP- Results showed mutation rate of p53 in metaplasia, dysplasia and gastric carcinoma was 37. 5 % (3/8), 42. 11 % (8/19), 53. 33 (16/30) respectively- There was significant dif-ference among groups of metaplasia, dysplasia, cancer and normal controls. Noexon8 mutation was found in metaplasia and dysplasia, but 4 cases were found to have exon8 mutation in cancer group. It is suggested that exon8 mutation occurs at the late stage of gastric cancer, but exon 5, 6, 7 mutation occur in the course ofprecancerous lesion to cancer. Loss of heterozygosity (LOH) of exon4, intron6,APC was 47,37 % (9/19), 8. 73% (2/23), 16. 67 % (3/18) respectively. LOH of exon4 had something to do with poor differentiation, lymph node metastasis,depth of invasion- LOH of exon4 may be one of prognostic marker of gastric cancer. We are led to conclude that p53 gene mutation is an early event and perhaps work together with ras oncogene in gastric carcinogenesis

APC and K-ras gene mutation in aberrant crypt foci of human colon

AIM To study the genetic alteration in ACF andto define the possibility that ACF may be a veryearly morphological lesion with molecularchanges, and to explore the relationshipbetween ACF and colorectal adenoma evencarcinoma.METHODS DNA from 35 CRC, 15 adenomas, 34ACF and 10 normal mucus was isolated by meansof microdissection. Direct gene sequencing of K-ras gene including codon 12, 13 and 61 as well asthe mutation cluster region (MCR) of APC genewas performed.RESULTS K-ras gene mutation frequency inACF, adenoma and carcinoma was 17.6% (6/34), 13.3% (2/ 15), and 14.3% (5/ 35)respectively, showing no difference ( P > 0.05)in K-fas gene mutation among three pathologicprocedures. The K-ras gene mutation inadenoma, carcinoma and 4 ACF restricted incodon 12 (GGT→GAT), but the other 2 mutationsfrom ACF located in codon 13 (GGC→GAC). K-res gene mutation was found more frequently inolder patients and patients with polypoidcancer. No mutation in codon 61 was found in thethree tissue types. Mutation rate of APO gene inadenoma and carcinoma was 22.9% (8/35) and26.7% (4/ 15), which was higher than ACF(2.9%) (P < 0.05). APC gene mutation incarcinoma was not correlated with age ofpatients, location, size and differentiation oftumor.CONCLUSION ACF might be a very earlymorphological lesion in the tumorogenesis ofcolorectal tumor. The morphological feature andgene mutation status was different in ACF andadenoma. ACF is possibly putative'microadenoma' that might be the precursor ofadenoma. In addition, the development of asubgroup of colorectal carcinomas mightundergo a way of 'normal epithelium→ ACF→carcinomas'.

Study of mutations of p53, APC and K-ras genes in 47 cases of intestinalmetaplasia of gastric mucosa

Objective:To study the role of the mutations of p53, APC and K-ras genes in 47 cases of 3 types of intestinal metaplasia (IM) of gastric mucosa. Methods:In 47 cases of IM, exons 5- 8 of p53 and exons 15 of APC were examined with PCR-SSCP and codon 12 of K-ras with PCR-RFLP to detect the existence of any mutations of these structures. Results:Muta- tions of p53, APC and K-ras were found in 29.8% (14/47),6.4% (3/47) and 6.4% (3/47) respectively in our series of patients who consisted of 33 with types I and II and 14 with type III of IM. The mutation rate of p53 was far higher in patients with type III IM (57.1%,8/14) than in those with types I and II IM(18.2%,6/33)(P <0.05). Though the mutation rate of APC and K-ras was also higher in the patients with type III IM than in those with types I and II IM, it was of no statistical significance (P >0.05). In one case of type III IM, mutation of both p53 and K-ras was found. Conclusion: The molecular changes of 3 types of IM are different. The mutation of p53 may be closely related to carcinogenesis in cases of type III IM and it serve as a sign for the early diagnosis of gastric carcinoma.

LOSS OF HETEROZYGOSITY INVOLVING THE APC TUMOR SUPPRESSOR GENE IN HUMAN COLORECTAL CARCINOMA

To investigate whether aberration of the APC gene play any role in the development of Chinese sporadic colorectal carcinomas,we used a polymorphic site located in exon 11 which creted a new restriction site for RsaI to analyze LOH for the APC gene.We found that 20/29(68.9%) patients with colorectal cancer were informative for the APC exon 11 site and loss of one allele was detected in 40% of 20 informativc cascs.These data suggested that loss of heterozygosity of APC gene(APC-LOH) play a role in the pathogenesis of Chinese colorectal cancer.APC-LOH is a earlier event of colorectal tumorigenesis and may be of diagnostic value in Patient suffering colorectal cancer.

Three Novel Mutations of APC Gene Found in a Chinese Family with Familial Adenomatous Polyposis

Objective:To identify the causative adenomatous polyposis coli(APC)gene defects associated with a pedigree of familial adenomatous polyposis(FAP).Methods:FAP was diagnosed based on clinical manifestations,family history,as well as endoscopic and pathological examinations.The blood samples of the FAP pedigree members,colonic polyp patients,and normal individuals were collected.Genomic DNA was then extracted from those samples.APC mutation analysis was conducted via direct polymerase chain reaction(PCR)sequencing.Results:Three synonymous mutations and a missense mutation were found:c.5034G>A(p.Glyl678Gly),c.5465T>A(p.Vall 822Asp),c.5880G>A(p.Prol960Pro),and c.5274T>G(p.Serl758Ser)・Among them,the homozygous mutation on APC gene c.5034G>A has been reported,while the other three mutations have not been reported in the Chinese Han population.Individuals with c.5465T>A(p.Vall822ASP)missense mutation eventually suffer from colon cancer and have poor prognosis.We found no mutation in patients with simple intestinal polyp and in normal individuals.In addition,there were homozygous and heterozygous mutations in different patients from the same family.Conclusion:Three new mutations of APC gene were firstly reported in Han population.The missense mutation of c.5465T>A(p.Vall 822Asp)may be the cause of carcinogenesis in this FAP pedigree with poor prognosis.

肺癌患者血清p16、FHIT、APC基因甲基化检测

目的:检测肺癌患者血清中抑癌基因p16、FHIT、APC的甲基化,探讨它们在肺癌发生和诊断中的临床价值。方法:收集120例原发性肺癌患者(肺癌组)、46例肺良性疾病患者(对照组)的血液标本,采用甲基化PCR方法检测2组患者血清p16、FHIT、APC基因甲基化。采用logistic回归分析肺癌发生的危险因素,计算上述基因甲基化诊断肺癌的准确率。结果:肺癌组血清中p16、FHIT、APC的甲基化率分别为37.5%、34.2%、31.7%,对照组中分别为6.5%、13.0%、10.9%,差异有统计学意义(P均<0.05)。Logistic回归分析提示p16、FHIT基因甲基化均为肺癌发生的独立危险因素,OR(95%CI)分别为7.509(2.160~26.099)、2.927(1.096~7.814)(P均<0.05)。p16、FHIT、APC基因甲基化单项诊断肺癌的准确率分别为53%、49%、47%,3种基因甲基化联合诊断肺癌的准确率为87%,优于单项指标。结论:p16、FHIT基因甲基化均为肺癌发生的独立危险因素;联合检测p16、FHIT、APC甲基化可提高肺癌诊断的准确性。

结直肠癌APC、K-ras、p53基因突变检测

目的:探讨结直肠癌中APC、K-ras、p53基因突变模式。方法:应用酚/氯仿法提取48例结直肠癌组织及其相应正常黏膜组织的DNA,用聚合酶链反应(PCR)、单链构象多态性分析(SSCP)和DNA测序等方法检测APC基因第15外显子突变密集区(mutation cluster region,MCR)区段、K-ras和p53基因的突变。结果:APC、K-ras和p53基因的突变率分别为37.5%(18/48)、43.8%(21/48)和35.4%(17/48)。48例结直肠癌组织中,有42例发生APC、K-ras或p53基因突变,突变率高达87.5%(42/48),其中仅有APC、K-ras或p53 1种基因发生突变的发生率分别为16.7%(8/48)、25.0%(12/48)和20.8%(10/48)。单独1种基因发生突变的总发生率为62.5%(30/48)。APC和p53,APC和K-ras或p53和K-ras 2种基因均有突变的发生率分别为6.3%(3/48)、10.4%(5/48)和4.2%(2/48)。APC、K-ras和p53 3种基因均发生突变的发生率为4.2%(2/48)。2种和3种基因均发生突变的总发生率为25%(12/48)。结论:结直肠癌的发生、发展并不完全遵循由正常结直肠黏膜上皮细胞向腺瘤和侵袭性癌转化的过程中,及依次发生“APC→K-ras→p53→DCC”突变累积这一经典的结直肠癌发生发展模式,可能存在其他结直肠癌发病机制。

痰标本FHIT、P16、MGMT、RASSF1A、APC基因甲基化在肺癌诊断中的作用

目的探讨肺癌患者痰标本中FH IT、P16、MGMT、RASSF1A和APC等抑癌基因启动子异常甲基化及其联合检测在肺癌筛查及早期诊断中的价值。方法采用甲基化特异性PCR(methylation specific PCR,MSP)法,检测47例肺癌组织及对应的痰标本FHIT、P16,MGMT、RASSF1A和APC基因启动子区甲基化状态。24例肺良性疾病患者痰标本作为对照。结果 47例肺癌组织标本中FHIT、P16、MGMT、RASSF1A、APC基因启动子区甲基化检出率分别为40.4%(19/47)、53.2%(25/47)、36.2%(17/47)、21.3%(10/47)和38.3%(18/47);对照的痰标本中五者甲基化检出率分别为38.3%(18/47)、48.9%(23/47)、36.2%(17/47)、17.0%(8/47)和29.8%(14/47),两组甲基化检出率存在着一致性[P>0.05;κ(0.8～1.0)]。24例肺良性病变痰标本中未检测到任何异常甲基化,与肺癌组比较差异有统计学意义(P<0.05)。五项指标联合检测可明显提高肺癌检测的灵敏度(80.9%)和特异度(100.0%)。FHIT和P16基因痰标本甲基化检出率与患者吸烟指数有相关性(P<0.05)。结论痰标本中多个肺癌相关基因甲基化联合检测有望成为肺癌筛查、早期诊断简便有效的指标。

大肠癌病人粪便和组织中APC基因突变的研究

[目的]探寻一种无创伤性的早期诊断大肠癌的方法。[方法]采用聚合酶链反应—单链构象多态性(PCR—SSCP)技术检测大肠肿瘤病人粪便脱落细胞和组织APC基因突变并加以分析比较。[结果]肿瘤组织突变率为44%(19/43)。患者粪便脱落细胞APC基因的突变率为37.75%(16/43),腺瘤和大肠癌APC基因突变分别为25%(2/8)和40%(14/35)。组织粪便APC基因突变率相比差异无统计学意义(χ2检验P﹥0.05)。两者一致性检验结果kappa值为0.8449,一致性极好。正常组织APC基因未发现有突变。[结论]在粪便能够检测出APC基因突变,且与组织检测到的突变一致性极好,所以大肠肿瘤粪便的APC基因检测有望成为大肠肿瘤早期诊断和人群筛检的最优方案。

宫颈癌APC基因启动子甲基化与其临床病理特征的关系

背景与目的:腺瘤性结肠息肉病(adenomatous polyposis coli,APC@基因是Wnt信号传导通路中重要的抑癌基因,其启动子区CpG岛高甲基化引起的基因失活可导致Wnt信号传导通路异常,与多种肿瘤有关。APC基因启动子甲基化与宫颈癌的关系研究较少。本研究检测宫颈癌标本中APC基因启动子甲基化状态,并分析其与临床病理特征及高危型人乳头瘤病毒(HPV@感染的关系,探讨APC基因启动子甲基化与宫颈癌的关系。方法:运用甲基化特异性PCR(MSP@检测95例宫颈癌标本及对照组20例正常宫颈组织的APC基因启动子甲基化状态,并分析APC基因甲基化状态与不同临床病理特征及高危型HPV感染之间的联系。结果:宫颈癌组APC基因甲基化率明显高于正常对照组(分别为56.8%,10%,P<0.01@。宫颈癌APC基因甲基化检测和高危型HPV DNA检测结果有较好的一致性(Kappa=0.348,P<0.001@。腺癌组甲基化率较鳞癌组高(分别为74.1%,50.0%,P<0.05@。APC甲基化阳性率随肿块增大及淋巴结转移而增高(P<0.05@。不同年龄、FIGO临床分期、WHO病理分级、肿瘤侵犯深度和APC基因甲基化未见明显关系(P>0.05@。结论:宫颈癌APC基因启动子甲基化与高危型HPV具有良好的一致性。APC基因启动子高甲基化为频发事件,并与不同宫颈癌病理类型相关,可作为宫颈癌诊断及分型的生物学标志物。

乳腺癌患者外周血清中APC基因启动子甲基化异常的检测及其意义

背景与目的:检测肿瘤患者外周血中肿瘤相关标志物是当前肿瘤研究的热点之一,恶性肿瘤患者外周血中存在游离的肿瘤相关DNA已引起肿瘤学界的极大关注,人们曾在多种肿瘤患者血清中发现与原发肿瘤相同的DNA变异。本研究以APC(adenomatouspolyposiscoli)基因启动子甲基化作为肿瘤标志物,探讨乳腺癌患者外周血清中游离的肿瘤相关DNA与肿瘤组织及临床病理参数的相关性。方法:采用甲基化特异性PCR(methylationspecific-PCR,MSP)方法分别检测84例乳腺癌组织、癌旁正常腺体组织及外周血清中游离DNAAPC基因启动子甲基化状况。结果:84例乳腺癌组织APC基因启动子甲基化频率为45.2%(38/84),相应外周血清中同样DNA变异阳性检出率为31.0%(26/84)。外周血清中DNA甲基化变异与肿瘤组织的甲基化状况显著相关(r=0.977,P0.002)。检测外周血清中APC基因甲基化的敏感性为68.4%,特异性为97.8%肿瘤组织及外周血清中游离DNA甲基化异常与临床分期、病理类型、肿块大小及受体状况无相关性(P>0.05)。肿瘤组织未检测到甲基化患者的血清中及健康人血清中均未检测到该基因甲基化变异。结论:乳腺癌患者外周血清中肿瘤相关DNA甲基化与肿瘤组织中相同基因的变异显著相关。

肺癌患者血浆中APC基因启动子甲基化定量检测研究

背景与目的:APC基因编码的蛋白参与信号转导途径,大量研究证实APC启动子区的高甲基化在肿瘤的发生发展中起重要作用。本研究建立血浆APC基因实时荧光定量甲基化特异性基因扩增(methylation-specificPCR,MSP)检测方法,并对临床肺癌患者血浆进行检测,以确定该方法在肺癌诊断中的应用价值。方法:将APC基因启动子甲基化阳性肺癌细胞株NCI-H460细胞用有限稀释法获取单个集落形成的细胞,以经典的酚-氯仿法提取细胞DNA,并用MSP对APC基因甲基化进行验证,紫外分光光度计定量并以10倍稀释的浓度梯度依次投入到200μL健康人血浆中,得到模拟肺癌患者血浆,利用磁珠核酸提取方法从模拟肺癌及肺癌患者、肺部良性疾病患者和健康对照者血浆中提取DNA,对血浆DNA模板进行亚硫酸氢盐化学修饰;以模拟血浆样品作为标准品,采用外标准曲线法对各种血浆样品中APC甲基化进行定量分析。结果:所建立的实时荧光定量MSP检测方法的线性范围为1.5×102～1.5×105拷贝/mL,用该方法检测甲基化肿瘤细胞的DNA其最低检测限为1.5×102拷贝/mL。78例肺癌患者有40例组织中检测出APC基因甲基化阳性,其中的19例(47.5%)肺癌患者血浆中APC基因启动子甲基化阳性,APC甲基化浓度为1.67×102～6.78×103拷贝/mL,中位浓度为1.60×103拷贝/mL。38例组织阴性的肺癌患者、31例肺部良性疾病患者和23例健康者的血浆APC基因启动子甲基化均为阴性。结论:实时荧光定量MSP检测血浆APC基因甲基化在肺癌诊断方面具有潜在应用价值。

Survivin shRNA和APC片段双基因的载体构建及其在HT-29细胞的表达

目的研究表明APC、Survivin 2种基因表达异常在结肠癌的发生发展中具有重要意义。构建Survivin shRNA、APC功能片段双基因共表达慢病毒载体并观察其能否于HT-29结肠癌细胞中成功表达,同时观察其是否能够对结肠癌细胞凋亡产生影响。方法构建3对互补Survivin shRNA片段,从其中筛选出一条最佳干扰shRNA片段,与APC功能片段(aa1020-1698)相连接构建双基因共表达质粒载体。将HT-29细胞分为实验组、空载组、空白组3组,慢病毒对HT-29进行侵染,观察是否有绿色荧光表达及对转染细胞进行realtime PCR、Western blot检测Survivin、APC基因表达水平。通过检测Caspase-3活性来检测细胞凋亡情况。结果 1Real time PCR检测后显示对Survivin基因起到最佳干扰效果的片段为shRNA3序列。2构建出的shRNA载体经过送序验证比对后,3对shRNA序列与最初设计的序列完全相同。在HT-29细胞中可见绿色荧光,实验组Survivin相对含量(31.71±1.49)较空载组(100±0)、空白组(95.12±2.15)明显减少(P<0.05),APC mRNA表达水平较空载组(0±0)、空白组(0.51±0.15)明显增加(P<0.05)。实验组Survivin蛋白相对含量(0.18±0.01)较空白组(0.24±0.04)、空载组(0.22±0.03)明显减少,APC蛋白表达水平(0.147±0.016)较空白组(0.095±0.012)、空载组(0.108±0.015)明显升高(P<0.05)。3实验组凋亡相对比值(0.573±0.050)较空白组(0.390±0.040)、空载组(0.407±0.030)明显增加(P<0.05)。结论成功构建Survivin-shRNA-APC双基因共表达慢病毒载体,并能够在HT-29结肠癌细胞中成功表达,该双基因共表达载体可为后续利用该载体进行基因治疗的基础实验提供材料。

散发性大肠癌组织及粪便P53蛋白、K-ras及APC基因的检测

目的了解大肠癌组织及粪便中P53蛋白K-ras及APC基因的突变状况,了解粪便脱落细胞基因检测的可行性及其临床意义方法采用S-P法对27例大肠癌患者的癌组织及其粪便脱落细胞 P53蛋白进行检测,以22例大肠癌组织及10倒粪便和9例正常大肠粘膜组织为研究对象,采用PCR-RFLP银染方法检测K-ras基因12,13密码子及应用PCR-SSCP银染技术检测APC基因突变集中区(MCR区)的突变状况结果粪便脱落细胞P53表达阳性率为37％(10/27),与相应患者大肠癌组织P53检测一致率为85％(23/27)、K-ras12密码子突变检出敏感性癌组织为73％(16/22),粪便为50％(5/10).粪便与相应患者的癌组织检测符合率为90％(9/10);癌组织及粪便中均未检出K-ras13密码子突变.癌组织中APC基因突变率为41％(9/22),粪便中APC突变体阳性检出率为40％(4/10),癌组织与相应患者的粪便APC基因检测一致率为90％(9/10).P53,K-ras及APC三个基因联合检测癌组织敏感性为100％,粪便为90％.结论 P53,K-ras及APC基因突变为散发性大肠癌常见的分子事件,联合基因检测可提高对大肠癌检测的敏感性;粪便中基因突变体检测结果忠实反映了癌组织突变状况,对其检测有望成为大肠癌诊断及筛查的无创分子途径.

家族性腺瘤性息肉病患者APC基因胚系突变的初步研究

目的:探讨国人家族性腺瘤性息肉病(FAP)患者APC基因胚系突变的特点。方法:对我院2004年3月至2005年3月收治的6例FAP患者运用PCR-变性高效液相色谱技术检测APC基因,对可疑突变者进行测序。结果:变性高效液相色谱检测共发现3个可疑突变片段,经DNA测序证实3个片段均存在突变。其中,15号外显子2例,14号内含子1例。结论:国人FAP患者相同基因型APC基因突变可有不同表现型。

SurvivinshRNA-APC双基因共表达慢病毒载体对HT-29结肠癌细胞裸鼠皮下移植瘤生长情况的影响

目的在转录后水平进行干预的RNA干扰技术在多基因治疗中的应用越来越广泛。文中旨在构建人HT-29结肠癌细胞裸鼠皮下移植瘤模型,通过联合RNAi和外源性补充的方式研究Survivin shRNA-APC双基因共表达慢病毒载体对结肠癌裸鼠移植瘤生长情况的影响。方法选取35只裸鼠随机数字表法分为5组,即Survivin shRNA-APC双基因组、Survivin shRNA组、APC组、空载组和空白组,每组7只;将已经构建好的处于对数生长期的双基因共表达Survivin shRNA-APC、Survivin shRNA及APC稳转株,空载稳转株,HT-29结肠癌细胞(均为2×106/mL)分别注射至5组裸鼠左前腋下成瘤,构建人HT-29结肠癌细胞裸鼠皮下移植瘤模型;通过测量瘤体体积、重量,检测移植瘤生长抑制率,Real time PCR检测移植瘤组织survivin mRNA的表达,免疫组化检测Survivin蛋白的表达,TUNEL检测凋亡情况。结果与空白组比较,APC组、Survivin shRNA组、双基因组移植瘤平均体积、平均重量均减少(P<0.05);与空载组比较,APC组、Survivin shRNA组、双基因组平均体积、平均移植瘤重量亦减少(P<0.05),而体积抑制率、瘤重抑制率均增加(P<0.05);与双基因组比较,APC组、Survivin shRNA组移植瘤平均体积、平均重量均增加(P<0.05)。与空白组和空载组相比,APC组、Survivin shRNA组、Survivin shRNA-APC双基因组移植瘤组织Survivin mRNA和蛋白表达相对含量明显降低(P<0.05);与Survivin shRNA组、APC组相比,双基因组移植瘤组织Survivin mRNA和蛋白表达相对含量亦明显降低(P<0.05)。与空白组裸鼠移植瘤组织结肠癌细胞凋亡指数[(9.89±0.31)%]比较,APC组、Survivin shRNA组、双基因组[(31.19±1.79)%、(33.64±2.03)%、(56.72±3.17)%]明显升高(P<0.05),而APC组、Survivin shRNA组、双基因组亦较空载组[(10.06±0.43)%]明显升高(P<0.05);与Survivin shRNA组、APC组相比,Survivin shRNA-APC双基因组移植瘤组织癌细胞凋亡指数明显升高(P<0.05)。结论 Survivin shRNA-APC双基因共表达慢病毒载体能够使Survivin基因的表达水平降低,促进结肠癌细胞的凋亡,抑制移植瘤的生长,且优于单个基因的影响。