Killing effect of TNF-related apoptosis inducing ligand regulated by tetracycline on gastric cancer cell line NCI-N87

AIM: To clone the cDNA fragment of human TRAIL (TNF-related apoptosis inducing ligand) into a tetracycline-regulated gene expression system, the RevTet-On system, transduce expression vectors into a gastric carcinoma cell line-NCI-N87 and examine the effects of controlled expression of TRAIL in vitro on the gastric carcinoma cells. METHODS: The full-length cDNA of TRAIL was inserted into a vector under the control of the tetracycline-responsive element (TRE) to obtain the plasmid pRevTRE-TRAIL, which was transfected into a packaging cell line PT67. In addition, vector pRev-Tet On and pRevTRE were also transfected into PT67 separately. After hygromycin and G418 selection, the viral titer was determined. The medium containing retroviral vectors was collected and used to transduce a gastric carcinoma cell line NCI-N87. The resulting cell line NCI-N87-Tet On TRE-TRAIL and a control cell line, NCI-N87 Tet On-TRE, were established. TRAIL expression in the cell line was induced by incubating cells with doxycycline (Dox), which is a tetracycline analogue. The killing effect on gastric carcinoma cells was analyzed after induction. RESULTS: The recombinant plasmid pRev-TRE-TRAIL was constructed. After hygromycin or G418 selection, the producer cell lines PT67-TRE, PT67-TRE-TRAIL and PT67-Tet On were obtained,with titers of about 10(8)CFU.L(-1). By transducing NCI-N87 cells with retroviral vectors from these cell lines, stable cell lines NCI-N87-Tet-On TRE-TRAIL (NN3T) and control cell line NCI-N87-Tet-On-TRE (NN2T) were established. The growth curves of the selected cell lines were the same with the wild type NCI-N87. When Dox was added, cell death was obvious in the test groups (29%-77%), whereas no difference was observed in control and wild type cell lines. With the addition of a medium from the test group, human leukemia cell line Jurkat was activated till death (83%), indicating the secretion of active TRAIL proteins from the test cells to the medium. CONCLUSION: With the use of the RevTet-On system, a regulated expression system for TRAIL was constructed. Using this system, the selected killing effect of TRAIL on gastric carcinoma cell line NCI-N87 could be observed.

Effects of Human Cytomegalovirus Infection on Apoptosis and Expression of Apoptosis-Regulating Factors

Summary： The present study aimed to find out dynamic changes of apoptosis in human cytomegalovirus （HCMV） infected cells and the influence of HCMV infection on activation of caspase-3 and the expression of apoptosis-regulating genes, bcl-2 and fas mRNA. The sequential changes of apoptotic cell rate in high and low MOI （MOI=2.5 and 0.25 respectively） of HCMV infected human embryonic lung fibroblasts （HELFs） at 1 h, 12 h, 24 h, 36 h, 48 h, 72 h and 96 h post-infection were measured by flow cytometry. The expression levels of caspase-3 protein and bcl-2 and fas mRNA in HCMV infected cells （MOI=0.25） at 72 h post-infection were detected by Western blot and in situ hybridization methods, respectively. It was found that the ratio of apoptotic cells in normal controls was consistently lower, but the rates in low and high MOI infected cells were gradually increased with time prolonged, reached peak at 96 h （8.85 %） and 72 h （25.63 %）, respectively. By Western blot analysis, only a narrow band of 32 kD （1 kD=0. 992 1 ku） procaspase-3 was found in normal cells, but a wider procaspase-3 band and a much wider band of 17 kD proteins （p17） ap- peared in the infected cells. Meanwhile, the expression of bcl-2 mRNA was higher and that of fas mRNA was lower in the normal HELF cells, whereas there were significantly lower bcl-2 mRNA and higher fas mRNA expression levels in HCMV infected cells. It was concluded that HCMV was a stronger inducer of apoptosis in HELF cells. Caspase-3, as the marker of undergoing apoptosis, was expressed increasingly and activated in the infected cells, indicating its action in HCMV-inducing apoptosis. Down-regulating bcl-2 mRNA expression and up-regulating fas mRNA expression were also involved in the mechanism of HCMV-induced apoptosis.

Bcl-2 over-expression and activation of protein kinase C suppress the Trail-induced apoptosis in Jurkat T cells

Trail, a tumor necrosis factor-related apoptosis-inducing ligand, is a novel potent endogenous activator of the cell death pathway through the activation of cell surface death receptors Trail-R1 and Trail-R2. Its role, like FasL in activation-induced cell death (AICD), has been demonstrated in immune system. However the mechanism of Trail induced apoptosis remains unclear. In this report, the recombinant Trail protein was expressed and purified. The apoptosis-inducing activity and the regulation mechanism of recombinant Trail on Jurkat T cells were explored in vitro. Trypan blue exclusion assay demonstrated that the recombinant Trail protein actively killed Jurkat T cells in a dose-dependent manner. Trail-induced apoptosis in Jurkat T cells were remarkably reduced by Bcl-2 over expression in Bcl-2 gene transfected cells. Treatment with PMA (phorbol 12-myristate 13-acetate), a PKC activator, suppressed Trail-induced apoptosis in Jurkat T cells. The inhibition of apoptosis by PMA was abolished by pretreatment with Bis, a PKC inhibitor. Taken together, it was suggested that Bcl-2 over-expression and PMA activated PKC actively down-regulated the Trail-mediated apoptosis in Jurkat T cell.

The involvement of p38 MAPK in transforming growth factor β1-induced apoptosis in murine hepatocytes

We reported in this manuscript that TGF-beta1 induces apoptosis in AML12 murine hepatocytes, which is associated with the activation of p38 MAPK signaling pathway. SB202190, a specific inhibitor of p38 MAPK, strongly inhibited the TGF-beta1-induced apoptosis and PAI-1 promoter activity. Treatment of cells with TGF-beta1 activates p38. Furthermore, over-expression of dominant negative mutant p38 also reduced the TGF-beta1-induced apoptosis. The data indicate that the activation of p38 is involved in TGF-beta1-mediated gene expression and apoptosis.

Relationship between Fas/ FasL expression and apoptosis of colon adenocarcinoma cell lines

INTRODUCTIONFas/ FasL system has been identified as a keymediator of apoptosis in tumor cells[1-4]. Theoccurrence and development of neoplasm are closelyrelated to apoptosis[5-7] Most chemotherapeuticdrugs kill cancer cells mainly by inducingapoptosis[8-14].'

Altered expression of nuclear matrix proteins in etoposide induced apoptosis in HL-60 cells

The events of cell death and the expression of nuclear matrix protein (NMP) have been investigated in a promyelocytic leukemic cell line HL-60 induced with etoposide. By means of TUNEL assay, the nuclei displayed a characteristic morphology change, and the amount of apoptotic cells increased early and reached maximun about 39% after treatment with etoposide for 2 h. Nucleosomal DNA fragmentation was observed after treatment for 4 h. The morphological change of HL-60 cells, thus, occurred earlier than the appearance of DNA ladder. Total nuclear matrix proteins were analyzed by 2-dimensional gel electrophoresis. Differential expression of 59 nuclear matrix proteins was found in 4 h etoposide treated cells. Western blotting was then performed on three nuclear matrix acssociated proteins, PML, HSC70 and NuMA. The expression of the suppressor PML protein and heat shock protein HSC70 were significantly upregulated after etoposide treatment, while NuMA, a nuclear mitotic apparatus protein, was down regulated. These results demonstrate that significant biochemical alterations in nuclear matrix proteins take place during the apoptotic process.

Thyroid hormone regulation of apoptotic tissue remodeling during anuran metamorphosis

Anuran metamorphosis involves systematic transformations of individual organs in a thyroid hormone (TH)-dependent manner. Morphological and cellular studies have shown that the removal of larval or- gans/tissues such the tail and the tadpole intestinal epithelium is through programmed cell death or apop- tosis. Recent molecular investigations suggest that TH regulates metamorphosis by regulating target gene expression through thyroid hormone receptors (TRs), which are DNA-binding transcription factors. Cloning and characterization of TH response genes show that diverse groups of early response genes are induced by TH. The products of these TH response genes are believed to directly or indirectly affect the expression and/or functions of cell death genes, which are conserved at both sequence and function levels in different animal species. A major challenge for future research lies at determining the signaling pathways leading to the activation of apoptotic processes and whether different death genes are involved in the regulation of apoptosis in different tissues/organs to effect tissue-specific transformations.

Molecular aspects of carcinogenesis in pancreatic cancer

BACKGROUND:Pancreatic cancer(PCa)is one of the most aggressive human solid tumors,with rapid growth and metastatic spread as well as resistance to chemotherapeutic drugs,leading rapidly to virtually incurable disease.Over the last 20 years,however,significant advances have been made in our understanding of the molecular biology of PCa,with a focus on the cytogenetic abnormalities in PCa cell growth and differentiation. DATA SOURCES:A MEDLINE search and manual cross- referencing were utilized to identify published data for PCa molecular biology studies between 1986 and 2008, with emphasis on genetic alterations and developmental oncology. RESULTS:Activation of oncogenes,deregulation of tumor suppressor and genome maintenance genes,upregulation of growth factors/growth factor receptor signaling cascade systems,and alterations in cytokine expression,have been reported to play important roles in the process of pancreatic carcinogenesis.Alterations in the K-ras proto- oncogene and the p16INK4a,p53,FHIT,and DPC4 tumor suppressor genes occur in a high percentage of tumors. Furthermore,a variety of growth factors are expressed at increased levels.In addition,PCa often exhibits alterations in growth inhibitory pathways and evades apoptosis through p53 mutations and aberrant expression of apoptosis-regulating genes,such as members of the Bcl family.Additional pathways in the development of an aggressive phenotype,local infiltration and metastasis are still under ongoing genetic research.The present paper reviews recent studies on the pathogenesis of PCa,and includes a brief reference to alterations reported for other types of pancreatic tumor. CONCLUSIONS:Advances in molecular genetics and biology have improved our perception of the pathogenesis of PCa.However,further studies are needed to better understand the fundamental changes that occur in PCa,thus leading to better diagnostic and therapeutic management.

缺血预处理对肝缺血再灌注时细胞凋亡及调控基因表达的影响

目的探讨缺血预处理对肝脏细胞凋亡的影响以及与调控基因bcl-2/bax蛋白表达的关系。方法将家兔分为假手术(SO)组、缺血再灌注(IR)组,缺血预处理(IP)组。后2组中再分为4个亚组(IR3h、12h、24h和48h组,IP3h、12h、24h和48h组)。缺血期均为60min。缺血预处理为缺血前采用5min缺血及5min再灌注的方法。分别于再灌注3、12、24和48h后处死动物采取肝脏标本,SO组于手术后24h采取肝标本。检测细胞凋亡及bc1-2/bax蛋白表达水平。结果IR组和IP组与SO组比较,细胞凋亡指数(AI)增加差异有显著性(P<0.01);IP组中IP3h、12h和24h较同时间段IR组细胞凋亡指数降低差异有显著性(P<0.05);bcl-2蛋白表达:IP组与IR组及SO组比较,增高差异有显著性(P<0.05);bax蛋白表达:IR组和IP组与SO组比较增加差异有显著性(P<0.05)。结论缺血预处理可能通过激活bcl-2蛋白的表达,改变bcl-2/bax表达比例从而抑制肝细胞凋亡。

双氢青蒿素对Lewis肺癌小鼠的抑瘤作用及其机制探讨

目的探讨双氢青蒿素对Lewis肺癌小鼠的抑瘤效应及其作用机制。方法C57BL/6J小鼠皮下接种3LL细胞(2×106)50只,随机分为5组,分别为生理盐水组、阳性对照顺铂组、双氢青蒿素高、中、低剂量组,检测各组小鼠的体重变化和抑瘤率,应用流式细胞术进行TUNEL分析和凋亡相关基因及其表达改变的检测。结果双氢青蒿素中、高剂量组体重较生理盐水组增加明显,其抑瘤率分别为53.5%及59.2%;流式细胞术TUNEL检测结果显示,其作用细胞凋亡和坏死同时存在。FCM法分析其对肺癌组织凋亡相关基因检测表明中、高剂量组Fas、p53等凋亡基因上调,Bcl-2抑制凋亡基因下调。结论双氢青蒿素对Lewis肺癌小鼠肺癌生长具有一定的抑制作用,能促进肿瘤细胞凋亡,其机制可能与调控细胞凋亡相关基因的表达有关。

细胞凋亡调控的分子机制(综述)

凋亡是细胞的主动死亡过程 ,在细胞的发育和疾病的发生中起重要的作用 ,涉及凋亡这一过程的因素众多 ,本文对近年来其中的一些因素如IEG、ICE、Fasl -Fas/Apo - 1(CD95)、Ca2 + 、ROS和NF -κB等对细胞凋亡的影响及其调控进行了综述。

细胞凋亡机制概述

细胞凋亡是一种重要的生物学过程,是在基因调控下所发生的一系列细胞主动死亡过程。就近几年细胞凋亡信号传递机制、酶学机制以及基因调控机制的研究作一概述。

含AFP基因调控序列的pAFP-P53-EGFP质粒诱导AFP阳性肝癌细胞凋亡

目的:观察含AFP基因调控序列的载体对AFP阳性肝癌细胞的靶向致凋亡作用。方法:将AFP启动子、沉默子和远端增强子Ⅲ组合为1.2 kb的AFP基因调控序列,构建pAFP-EGFP载体,分别转染人肝癌HepG2(AFP阳性)、人肝癌SMMC7721(AFP阴性)和人宫颈癌HeLa(AFP阴性)细胞,荧光显微镜下观察EGFP荧光蛋白表达强度。引入P53基因片段,构建pAFP-P53-EGFP重组质粒,转染HepG2、SMMC7721和HeLa细胞,Western blotting检测各组细胞P53蛋白的表达,流式细胞术分析各组细胞凋亡率及细胞周期。结果:成功构建了pAFP-EGFP和pAFP-P53-EGFP重组质粒。pAFP-EGFP转染后,AFP阳性的HepG2细胞中EGFP荧光蛋白表达显著高于AFP阴性的SMMC7721和HeLa细胞。pAFP-P53-EGFP转染后,HepG2细胞中P53蛋白的表达量明显高于SMMC7721和HeLa细胞;HepG2细胞的G1期细胞及细胞凋亡率明显高于SMMC7721和HeLa细胞[(66.7±0.25)%vs(50.5±0.18)%,(51.0±0.20)%,P<0.05;(2.65±0.08)%vs(0.42±0.03)%,(0.39±0.02)%,P<0.05],但S期细胞明显低于转染后SMMC7721和HeLa细胞[(20.1±0.22)%vs(29.8±0.18)%,(37.8±0.21)%,P<0.05]。结论:含AFP基因调控序列的pAFP-P53-EGFP载体可专一性地作用于AFP阳性肝癌细胞,引起肝癌细胞周期阻滞和凋亡。

天然药物诱导细胞凋亡的研究进展

Apoptosis,a form of cell death,has generated considerable interest in recent years.Much progress has been made on the apoptosis induced by natural drgus,including component or mixture of plant,animal,mineral or marine materials,This review discusses some of the natural drugs that induce apoptosis and the possible mechanisms.

补肾及健脾复方对皮质酮大鼠T细胞凋亡信号相关基因群调控模式的对比研究

目的:探讨补肾及健脾复方对皮质酮大鼠T细胞凋亡信号相关基因表达的调控模式。方法:采用TUNEL标记的流式细胞技术,对皮质酮大鼠模型及各治疗组激活诱导的T细胞凋亡进行定量分析;采用荧光实时定量PCR技术对各组大鼠T细胞凋亡信号相关基因群mRNA表达水平进行定量与比较;采用分光光度法检测caspase-8、caspase-3的活性。结果:(1)与正常组相比,模型组T细胞凋亡百分率明显增高;右归饮组及补肾益寿胶囊组T细胞凋亡百分率与皮质酮模型组相比明显降低;四君子汤与模型组相比T细胞凋亡百分率无显著性差异。(2)模型组促凋亡的Fas、FasL、TNR1、Bax基因表达上调,抗凋亡的TNFR2、Bcl-2、cIAP1、cIAP2基因表达下调;两个补肾复方均可下调FasL、TNFR1mRNA表达水平,并可上调Bcl-2、cIAP1、cIAP2mRNA表达水平;四君子汤仅对Bcl-2,cIAP2mRNA表达水平有显著上调作用。(3)模型组caspase-8、caspase-3活性显著增高,两个补肾复方均可降低caspase-8、caspase-3的活性,四君子汤对caspase-8、caspase-3的活性无显著下调作用。结论:两个补肾复方下调促凋亡基因FasL、TNFR1的转录,上调抗凋亡基因Bcl-2、cIAP1、cIAP2的转录,并且降低caspase-8、caspase-3的活性,从而降低皮质酮大鼠过度的T细胞凋亡,是补肾法特有的对皮质酮大鼠T细胞凋?

缺血预处理对鼠肝细胞凋亡及调控基因(bcl-2,Fas)蛋白表达的影响

目的 观察鼠肝缺血再灌注损伤对肝细胞凋亡 ,以及缺血预处理对缺血再灌注损伤引起的肝细胞凋亡以及对其调控基因 (bcl 2 ,Fas)蛋白表达的影响。方法 Wistar大鼠分为假手术 (SO)组、缺血再灌注 (IR )组、缺血预处理 (IP)组 ,后 2组中分为 3个亚组 (IR1,2 ,3 ,IP1,2 ,3)。缺血均为 30min。缺血预处理为缺血前采用 5min缺血及 5min再灌。分别于再灌注1 5 ,3 ,4 5h后处死动物采取肝脏标本 ,SO组于术后 3 5h采取肝标本。检测细胞凋亡及bcl 2 ,Fas蛋白表达水平。结果 IR2 组和IP2 组与SO组比较细胞凋亡指数 (AI)显著性增加 (P<0 .0 1) ,IP组较IR组细胞AI显著性降低 (P <0 .0 5 )。电镜示凋亡细胞 ,但IP组较IR组的细胞器特别是线粒体损伤要轻。bcl 2蛋白表达 :IP组较IR组及SO组显著性增加 (P <0 .0 5 ) ,IR组与SO组无差异 (P >0 .0 5 )。Fas蛋白表达 :IR2 组和IP2 组较SO显著性增高 (P <0 .0 5 ) ,IP组与IR组比较无显著性差异 (P >0 .0 5 )。结论 IR损伤可能通过激活Fas蛋白的表达而促发肝细胞凋亡 ;IP可能通过激活bcl

超声介入复方中药“99-克星”活性组分诱导肝癌细胞凋亡及机制

目的探讨超声引导瘤内注射用复方中药“99-克星”的活性组分AG-05诱导体外培养肝癌HepG2细胞凋亡作用及相关机制。方法不同浓度AG-05作用于体外培养肝癌HepG2细胞后,应用荧光显微镜观察细胞形态学改变,流式细胞术分析细胞凋亡率变化,Westernblotting方法检测细胞bcl-2、caspase-3蛋白表达的改变。结果AG-05作用48h后肝癌HepG2细胞出现染色质边集、凋亡小体形成等典型的凋亡形态学改变,细胞凋亡率明显升高,10、20μg/ml组分别为(13.5±2.1)%和(20.1±4.3)%;AG-05具有抑制肝癌细胞bcl-2表达,活化caspase-3的作用,并且呈一定的量效、时效关系。结论复方中药“99-克星”活性组分AG-05可诱导肝癌细胞凋亡,其作用机理与抑制bcl-2蛋白表达,活化caspase-3有关。

大蒜新素对人巨细胞病毒感染的人胚肺成纤维细胞凋亡的影响

目的研究大蒜新素对人巨细胞病毒(HCMV)诱导感染的人胚肺成纤维细胞(HELF)凋亡的动态变化及凋亡调控基因bcl-2和fasmRNA表达的影响。方法用流式细胞术测定HELF在高、低感染复数(MOI分别为2.5、0.25)HCMV感染后1、12、24、36、48、72、96h凋亡细胞比率;大、中、小剂量大蒜新素(9、6和3μg/mL)处理正常的和感染的HELF细胞(MOI为2.5)后上述各时间点凋亡细胞比率。用原位杂交法检测大剂量大蒜新素处理感染细胞(MIO为0.25)72h后bcl-2和fasmRNA表达强度变化,并与正常细胞和感染细胞对比分析。结果正常细胞凋亡比率保持恒定低水平(凋亡率平均2.68%);低、高感染复数感染细胞随时间延长凋亡细胞逐渐增多,凋亡率峰值分别达8.85%(96h)和25.63%(72h);各剂量大蒜新素处理的正常细胞凋亡率增加,呈剂量依赖性,峰值分别为4.88%、6.47%和8.35%;但各剂量药物处理感染细胞后却使细胞凋亡比率下降,大剂量药物处理72h时效应最为明显,凋亡细胞比率由25.63%降至16.24%。正常细胞高表达bcl-2,低表达fas基因;感染HCMV后,bcl-2表达显著下调,fas表达明显增强;大蒜新素处理感染细胞后使bcl-2表达强度明显高于感染细胞,fas表达水平明显低于感染细胞,但仍未恢复到正常细胞水平。结论HCMV是HELF凋亡的强诱导剂;

大鼠肝纤维化模型中肝细胞凋亡及其调控基因的表达

目的观察肝细胞凋亡及其调控基因在肝纤维化形成过程中的动态变化,探讨其在肝纤维化发病机制中的作用。方法雄性Wistar大鼠28只(体质量85g～95g)随机分为4组。A,B,C为实验组,采用腹腔注射CCl_4的方法造模;D为对照组,代之以生理盐水。于2,4,6wk末分别处死A,B,C三组大鼠,D组同期处理。取肝脏石蜡包埋,连续切片做HE染色、细胞凋亡原位TUNEL检测、BAX,BCL-X_L蛋白S-P法免疫组化染色。结果 HE染色A,B,C三组分别符合肝纤维化的Ⅰ,Ⅲ,Ⅳ期,凋亡的肝细胞在肝组织中散在分布TUNEL检测各实验组(A,B,C)肝细胞凋亡级数均高于对照组(D)(2.5±0.6),(2.8±0.4),(2.0±0.6)vs(0.3±0.5),(P<0.01,q_(AD)=9.86,q_(BD)=11.36,q_(CD)=7.59).S-P法免疫组化检测BAX,BCL-X_L主要分布于中央静脉及肝细胞坏死灶周围,在各实验组(A,B,C)中的表达强度均高于对照组(D)。BAX:(1.0±0.6),(1.5±0.6),(1.2±0.4)vs(0.3±0.5),(P<0.05,q_(AD)=3.05,q_(CD)=3.82,A,CvsD;P<0.01q_(BD)=5.32,BvsD)。BCL-X_L:(1.5±0.6),(1.3±0.8),(1.8±0.4)vs(0.3±0.5),(P<0.01,q_(AD)=4.88,q_(BD)=4.16,q_(CD)=6.25,A,B,CvsD)。各实验组的BAX/BCL-X_L高于对照组((0.9+0.8),(2.2±1.2),(0.6±0.4)vs(0.4±0.2),(P<0.05,q_(AD)3.44,q_(BD)=3.40,A,CvsD;P<0.01,q_(BD)=5.14,BvsD)。凋亡级数与BAX/BCL-X_L呈正相关(r=0.60137,P<0.05)。结论肝细胞凋亡在肝纤维化发生过程中存在动态变化,凋亡调控基因bax,bcl_x_1的表达及其比率是变化的主要原因之一。

钟基因Per2对白血病K562细胞增殖、分化、凋亡的影响及其机制研究

目的研究钟基因Period2(Per2)对慢粒急变K562细胞株增殖、分化、凋亡的影响及可能的分子机制。方法将Per2表达质粒pcDNA3.1-Per2及空载对照质粒pcDNA3.1分别经阳离子脂质体介导转染K562细胞,用G418筛选出Per2稳定表达细胞株。瑞氏染色观察细胞形态,台盼蓝拒染法和MTT法检测K562细胞增殖,流式细胞仪分析细胞周期和凋亡,电镜观察细胞凋亡,RT-PCR及Western blot方法检测该细胞株中增殖、凋亡相关基因p53、cyclin B1和c-myc等的表达。结果筛选到稳定表达Per基因的稳定表达细胞株K562/Per2细胞,与空载体转染组及未处理对照组细胞相比,K562/Per2细胞体积缩小,但是分化不明显;台盼蓝拒染法和MTT实验发现Per2抑制细胞生长与增殖能力;流式细胞仪检测周期结果K562/Per2细胞中G2期细胞增多[转染组(36.1±5.5)%,空载组(12.5±2.9)%,未处理对照组(9.7±2.3)%,P<0.05],凋亡检测显示转染组细胞凋亡明显增加[14.8%P<0.05];电镜结果显示染色质浓集、断裂,核固缩和凋亡小体;RT-PCR及Western blot显示Per2明显上调p53基因的mRNA和蛋白表达,而抑制cyclin B1、c-myc基因mR-NA和蛋白的表达。结论钟基因Per2能抑制K562细胞的生长和增殖,并诱导其发生凋亡,但对分化无明显作用。其机制可能是通过对细胞周期相关基因的调控并阻止细胞周期进程来实现的。