CDK5

摘要： Neurodegenerative diseases are caused by the progressive loss of specific neurons.The exact mechanisms of action of these diseases are unknown,and many studies have focused on pathways related to abnormal accumulation and processing of proteins,mitochondrial dysfunction,and oxidative stress leading to apoptotic death.However,a growing body of evidence indicates that aberrant cell cycle re-entry plays a major role in the pathogenesis of neurodegeneration.The activation of the cell cycle in mature neurons could be promoted by several signaling mechanisms,including c-Jun N-terminal kinases,p38 mitogen-activated protein kinases,and mitogen-activated protein kinase/extracellular signal-regulated kinase cascades;post-translational modifications such as Tau-phosphorylation;and DNA damage response.In all these events,implicated Cdk5,a proline-directed serine/threonine protein kinase,seems to be responsible for several cellular processes in neurons including axon growth,neurotransmission,synaptic plasticity,neuronal migration,and maintenance of neuronal survival.However,under pathological conditions,Cdk5 dysregulation may lead to cell cycle re-entry in post-mitotic neurons.Thus,Cdk5 hyperactivation,by its physiologic activator p25,hyper-phosphorylates downstream substrates related to neurodegenerative diseases.This review summarizes factors such as oxidative stress,DNA damage response,signaling pathway disturbance,and Ubiquitin proteasome malfunction contributing to cell cycle re-entry in post-mitotic neurons.It also describes how all these factors are linked to a greater or lesser extent with Cdk5.Thus,it offers a global vision of the function of cell cycle-related proteins in mature neurons with a focus on Cdk5 and how this protein contributes to the development of Alzheimer’s disease,Parkinson’s disease,amyotrophic lateral sclerosis,and Huntington’s disease by cell cycle activation.

摘要： 目的:探究钙激活中性蛋白酶14(CAPN14)在口腔鳞癌(OSCC)中的生物学效应及作用机制。方法:生物信息学方法分析CAPN14在OSCC细胞系SCC9、SCC25和CAL27中的临床特征及相互作用分子,慢病毒转染技术将CAL27细胞分为对照组、CAPN14过表达组及回复组。实时荧光定量PCR(qPCR)及Western Blot检测CAPN14和CDK5的mRNA及蛋白表达;CCK-8实验检测细胞增殖能力;Transwell侵袭实验检测细胞侵袭能力。结果:相比癌旁组织,OSCC组织中CAPN14的表达含量下降(P<0.01)。相比对照组,过表达组CAL27细胞中CDK5的蛋白表达水平降低,CDK5蛋白半衰期缩短,细胞增殖及转移能力减弱(P<0.01);而相比过表达组,回复组细胞CDK5的蛋白表达水平增高,细胞增殖及转移能力增强(P<0.01)。结论:CAPN14可促进CDK5蛋白的降解,并抑制OSCC细胞的恶性增殖及转移能力。

摘要： 目的阐明高血糖诱导对阿尔兹海默症(Alzheimer’s Disease,AD)样病理改变的潜在分子机制。方法选取18周龄的Sprague Dawley(SD)大鼠30只,将其随机分为对照组(Control)、模型组(STZ+HFD)以及模型+AMPK激动剂AICAR(5-Aminoimidazole-4-carboxamide1-β-D-ribofuranoside)组(STZ+HFD+AICAR),每组均为10只大鼠。模型组在高脂饮食(High-Fat Diet,HFD)喂养的基础上,经腹腔注射的方式给予大鼠50 mg/kg链脲佐菌素(Streptozotocin,STZ)建立2型糖尿病(TypeⅡDiabetes Mellitus,T2MD)/高血糖模型,STZ+HFD+AICAR组另给予大鼠100 mg/kg的AICAR,Control组给予常规饲料喂养并给予等量的柠檬酸钠缓冲液腹腔注射作为对照。8周内连续测量大鼠空腹血糖,8周后对各组大鼠进行糖耐量检测。通过Morris水迷宫实验分析各组大鼠认知功能的变化。采用Western Blot方法检测三个实验组大鼠脑组织AMPK/SIRT1通路分子、CDK5和H3acK9的表达变化。脑组织免疫组织化学染色检测AD特征性分子病理蛋白MAPT/Tau的磷酸化活性。结果与Control组相比,8周高脂喂养联合STZ注射3天后,大鼠空腹血糖于第2周开始升高直至第8周(P<0.05),且8周后糖耐量显著受损(P<0.05),血清胰岛素水平显著升高(P<0.01)。STZ+HFD大鼠的水迷宫定位航行试验逃避潜伏时间明显延长(P<0.05),而水迷宫空间探索时间显著降低(P<0.05)。Western Blot结果显示,与Control组相比,STZ+HFD大鼠脑组织磷酸化的AMPK蛋白以及SIRT1蛋白的表达水平显著降低,而H3acK9和CDK5蛋白表达水平显著升高。脑组织免疫组织化学结果显示,Tau蛋白磷酸化水平显著升高。AICAR可部分改善脑组织分子病理改变,如:增加磷酸化AMPK蛋白以及SIRT1蛋白的表达,减少H3acK9和CDK5蛋白表达,进而降低Tau蛋白磷酸化水平。结论AMPK/SIRT1通路失活促进去乙酰化蛋白H3acK9及CDK5的表达,进而引起Tau蛋白活性增加,该机制是高血糖引起脑组织AD样分子病理改变的潜在机制之一。

摘要： Identification of regulators of osteoblastogenesis that can be pharmacologically targeted is a major goal in combating osteoporosis,a common disease of the elderly population. Here, unbiased kinome RNAi screening in primary murine osteoblasts identified cyclin-dependent kinase 5(Cdk5) as a suppressor of osteoblast differentiation in both murine and human preosteoblastic cells. Cdk5 knockdown by si RNA, genetic deletion using the Cre-lox P system, or inhibition with the small molecule roscovitine enhanced osteoblastogenesis in vitro. Roscovitine treatment significantly enhanced bone mass by increasing osteoblastogenesis and improved fracture healing in mice. Mechanistically, downregulation of Cdk5 expression increased Erk phosphorylation, resulting in enhanced osteoblast-specific gene expression. Notably, simultaneous Cdk5 and Erk depletion abrogated the osteoblastogenesis conferred by Cdk5 depletion alone, suggesting that Cdk5 regulates osteoblast differentiation through MAPK pathway modulation. We conclude that Cdk5 is a potential therapeutic target to treat osteoporosis and improve fracture healing.

摘要： 目的 研究TGF-β1调控Cdk5表达在人肾系膜细胞外基质沉积中的作用.方法 10μg·L-1的TGF-β1刺激体外培养的人肾小球系膜细胞(HMC),检测其对系膜细胞Cdk5、p35/p25表达的影响;转染Cdk5过表达质粒,Western blot、免疫荧光检测胶原蛋白FN、CollagenⅣ表达的变化;应用Cdk5激酶活性抑制剂Roscovitine或转染Cdk5干扰质粒,Western blot、Real time-PCR、免疫荧光检测抑制Cdk5对TGF-β1刺激HMC后FN、CollagenⅣ蛋白及mRNA表达的影响.结果 TGF-β1作用于HMC后,Cdk5、p35/p25蛋白及mRNA表达均呈时间依赖性增高;与正常对照组相比,转染Cdk5过表达质粒,FN、CollagenⅣ蛋白表达增加,FN(绿色荧光)、CollagenⅣ(红色荧光)增强;与TGF-β1刺激组相比,加用10μmol·L-1的Roscovitine或转染Cdk5干扰质粒,FN、CollagenⅣ蛋白及mRNA表达均减少,FN(绿色荧光)、CollagenⅣ(红色荧光)减弱,而空质粒转染组没有明显变化.结论 一定浓度的TGF-β1可诱导系膜细胞内Cdk5表达增加,抑制Cdk5可降低系膜细胞外基质沉积.

摘要： 目的 观察APPswe/PS1dE9双转基因阿尔茨海默病模型小鼠认知功能的变化,探讨其与海马细胞周期蛋白依赖性蛋白激酶5及其激动因子细胞周期蛋白(Cdk5/p25)表达的关系.方法 通过Morris水迷宫观察3、6、9月龄APPswe/PS1dE9双转基因小鼠和同种野生型小鼠学习记忆能力的变化;采用western blotting法及免疫组织化学染色法检测其海马内Cdk5/p25的表达水平.结果 通过Morris水迷宫训练发现,3月龄APPswe/PS1dE9双转基因小鼠学习记忆能力与同月龄野生型小鼠比较,差异无统计学意义(P>0.05);而6、9月龄APPswe/PS1dE9双转基因小鼠较同月龄野生型小鼠定位航行实验潜伏期逐渐延长,差异有统计学意义(P<0.05).Western blotting结果显示,6、9月龄APPswe/PS1dE9双转基因小鼠海马内Cdk5/p25的表达水平较同月龄野生型小鼠增高,差异均有统计学意义(P<0.05).免疫组织化学染色结果显示,6、9月龄APPswe/PS1dE9双转基因小鼠海马内Cdk5阳性细胞的表达与同月龄野生型小鼠比较,差异有统计学意义(P<0.05);且随着年龄的增长,APPswe/PS1dE9双转基因小鼠海马内Cdk5阳性细胞表达逐渐增多,差异有统计学意义(P<0.05).结论 APPswe/PS1dE9双转基因小鼠学习记忆能力的下降与Cdk5/p25活性异常表达有关.

摘要： 目的 观察沉默细胞周期蛋白依赖性激酶5(Cdk5)对星形胶质细胞活化增殖和细胞周期的影响.方法 培养及鉴定SD大鼠星形胶质细胞,设计合成针对星形胶质细胞Cdk5的小干扰RNA(siRNA),将Cdk5 siRNA转染入星形胶质细胞,通过Real-time PCR和Western blot检测沉默效率;分为对照组及Cdk5 siRNA干预组,在不同时间点(3、6、12及24 h)采用Edu染色及流式细胞术检测细胞增殖及细胞周期情况.结果 成功利用Cdk5 siRNA沉默星形胶质细胞Cdk5;Edu染色显示Cdk5 siRNA干预组干预3、6、12hEdu染色阳性率较对照组显著降低(P＜0.01);流式细胞术显示Cdk5 siRNA干预组干预3、6、12 h处于S期的星形胶质细胞比例较对照组显著降低(P＜0.05).结论 沉默Cdk5可抑制星形胶质细胞的增殖及细胞周期进展,提示Cdk5在星形胶质细胞增殖过程中起到重要作用.%Objective To observe the effect of Cyclin-dependent kinase5(Cdk5) konckdown by RNA interfering on astrocyte proliferation and cell cycle progression.Methods Astrocytes were cultured from SD neo nate rats and the purity of astrocytes were identified by immunofluorescence staining of glial fibrillary acidic protein.Cdk5 siRNA were designed and synthesized.Those siRNAs were tansfected into astrocytes via Lipofecttamine 2000 and the silence efficiency was counted by Real-time PCR and Western blot.Astrocytes were randomly divided into two groups:control group and Cdk5 siRNA group.At different time points (3 h,6 h,12 h and 24 h).Edu staining and flow cytometry were used to measure the proliferation and cell cycle of astrocytes.Results Specificity Cdk5 silencing on astrocytes could be established by Cdk5 siRNA sequence successfully.Edu staining showed that the percentage of Edu positive cells in Cdk5 siRNA intervention group was significantly lower than that in the control group at 3 h,6 h and 12 h after intervention (P＜0.01).flow cytometry showed that the percentage of astrocytes in S phase in Cdk5 siRNA intervention group was lower than that in the control group at 3h,6h and 12h after intervention (P＜0.05).Conclusion Knockdown of Cdk5 could inhibite the proliferation and cell cycle progression of astrocytes.It was suggested that Cdk5 might paly important roles in the proliferation of astrocytes.

摘要： 目的:研究细胞周期蛋白依赖性激酶(Cdk)5和p35在星形胶质细胞中的表达及缺血再灌注后的其表达变化趋势.方法:离体培养SD大鼠星形胶质细胞,通过免疫荧光染色观察Cdk5和p35在星形胶质细胞中的表达分布.对培养的星形胶质细胞进行糖氧剥夺/恢复(OGD/R)处理,Western blot检测Cdk5和p35在星形胶质细胞OGD/R后不同时间点的表达变化.结果:Cdk5和p35均在星形胶质细胞中存在表达,以胞浆为主,胞核表达较少;两者表达分布一致.OGD/R后Cdk5和p35的表达呈早期显著上升,后期下降的趋势.结论:Cdk5和p35在星形胶质细胞中均存在表达,以胞浆为主,且两者表达分布基本一致.OGD/R后星形胶质细胞中的Cdk5和p35的表达呈动态变化.%Objective: To investigate the expression of Cdk5 and p35 in primary cultured astrocytes and the changes in expression induced by ischemia/reperfusion. Methods: Astrocytes were cultured from SD neonate rats. The expression and distribution of Cdk5 and p35 in cultured astrocytes were analyzed by immunofluorescence staining. Primary cultured astrocytes were subjected to oxygen-glucose deprivation/reperfusion(OGD/R),and the changes in Cdk5 and p35 expression after OGD/R were observed by Western blot. Results:Cdk5 and p35 were expressed in astrocytes,mainly in the cytoplasm and less in the nucleus,and both displayed similar cellular distribution.The expression of Cdk5 and p35 in astrocytes was increased during early phases and decreased during late phases after OGD/R. Conclusion: Both Cdk5 and p35 were expressed in astrocytes, and both showed similar, mainly cytoplasmic distribution. Cdk5 and p35 expression in astrocytes exhibited dynamic changes after OGD/R.

摘要： Objective This study aims to evaluate the changes of Cdk5 expression at the time of 3 hours to 10 days after moderate brain injury by blunt force impact in a rat model,and to demonstrate its forensic significance.Methods To establish a rat model of blunt focal brain contusion,and to observe the changes of Cdk5 expression in brain tissue at different timepoints after brain injury by immunohistochemistry and Western blot.Results A low expression level of Cdk5 was observed in the brain tissue of both normal and sham control groups.The expression of Cdk5 increased after 3 and 6 hours,remarkably increased at 12 hours,and reached the maximal level at 24 hours after focal brain injury.The Cdk5 level gradually decreased 3 days,5 days,7 days,and 10 days and reached the normal level 7 and 10 days after the injury,with no statistical difference (P＞0.05) compared with the normal and sham control groups.Conclusion The expression of Cdk5 increased in the peripheral area of contusion tissue after blunt brain injury in rats,showing single peak change,and dropped to normal level with the time extension.The change of Cdk5 expression may provide a new reference index for the prediction of early brain contusion.%目的 研究大鼠受到一定钝力打击造成中度脑损伤后,3h至l0d脑组织Cdk5的表达规律及法医学意义.方法 建立大鼠钝力性局灶性脑挫伤模型,应用免疫组织化学技术和免疫蛋白印迹技术观察脑损伤后不同时间脑组织中Cdk5表达变化.结果 正常组、假手术组脑组织有少量Cdk5表达;实验组损伤后3h组、6h组Cdk5表达增高,12h组表达明显升高(P＜0.05);在24h达到峰值,3d组、5d组、7d组、10d组逐渐下降,并在7d组、10d组基本降至正常,与正常组、假手术组比较基本无差异性(P＞0.05).结论 大鼠钝力性脑挫伤后Cdk5在挫伤脑组织周边区表达量增多,并呈现单峰变化,随时间延长基本降至正常.Cdk5表达变化可为早期脑挫伤时间推断奠定基础,提供新的参考指标.

摘要： Objective To explore the mechanism of Puerarin in the treatment of peripheral nerve injury in rats. Methods The model of denervated skeletal muscle was made in 28 rats(230~250 g). The experimental animals were randomly divided into four groups. In the Puerarin treatment group, the rats were given intraperitoneal injection of 50 mg/kg puerarin after ciatic nerve transection, and the same dose was injected every 24 hours in the next two days. In Inhibitor pretreatment group, the rats were given the 30 mg/kg inhibitor by intravenous injection, 60 minutes before the denervated skeletal muscle model was made. After denervation for 60 minutes, reinjection for 48 hours, and then the apoptotic index and the activity of Cdk5 and p25 were detected. Results Denervation of skeletal muscle led to increased activity of Cdk5 and p25, and increased number of apoptotic cells. Puerarin can decrease the number of apoptotic cells and the activity of Cdk5 and p25. Conclusion The remission of denervated skeletal muscle atrophy is related to the inhibition of Cdk5 and p25. The inhibitory effect of Puerarin on Cdk5 and p25 is one of the neuroprotective mechanisms.%目的 探索葛根素在治疗大鼠周围神经损伤中的作用机制.方法 对28只体重在230~250 g的雄性大鼠制作失神经骨骼肌模型.实验动物随机分为四组.在葛根素治疗组中,对再灌注后-坐骨神经切断的大鼠给予50 mg/kg葛根素进行腹腔内注射,随后两天每24小时以同样的剂量注射.在抑制剂预处理组中,对大鼠制作失神经骨骼肌模型60 min之前给予30 mg/kg抑制剂进行静脉注射.失神经60 min后进行48 h的再灌注-注射,然后检测其细胞凋亡指数及Cdk5和p25的活性.结果 骨骼肌失神经,导致Cdk5和p25的活性升高、凋亡细胞数增多.葛根素可以降低细胞凋亡数及Cdk5和p25的活性.结论 失神经骨骼肌萎缩的缓解与Cdk5及p25受抑制相关,在失神经骨骼肌模型大鼠的治疗过程中,葛根素对Cdk5及p25的抑制作用是其神经保护性机制之一.

摘要： 疼痛及其治疗是临床上的一大难题,主要由于机制不明.Cdk5是一种特殊的细胞周期素依赖性激酶家族,几乎存在于整个中枢和外周神经系统的神经元内.Cdk5作为丝氨酸/苏氨酸激酶,可调节众多底物和蛋白,目前发现在疼痛信号通路及阿片耐受中具有重要作用,可能作为治疗疼痛的新方法,对其在疼痛通路及阿片耐受中作用的深入了解,将有助于解决这一难题.

摘要： 疼痛及其治疗是临床上的一大难题,主要由于机制不明.Cdk5是一种特殊的细胞周期素依赖性激酶家族,几乎存在于整个中枢和外周神经系统的神经元内.Cdk5作为丝氨酸/苏氨酸激酶,可调节众多底物和蛋白,目前发现在疼痛信号通路及阿片耐受中具有重要作用,可能作为治疗疼痛的新方法,对其在疼痛通路及阿片耐受中作用的深入了解,将有助于解决这一难题.

摘要： 疼痛及其治疗是临床上的一大难题,主要由于机制不明.Cdk5是一种特殊的细胞周期素依赖性激酶家族,几乎存在于整个中枢和外周神经系统的神经元内.Cdk5作为丝氨酸/苏氨酸激酶,可调节众多底物和蛋白,目前发现在疼痛信号通路及阿片耐受中具有重要作用,可能作为治疗疼痛的新方法,对其在疼痛通路及阿片耐受中作用的深入了解,将有助于解决这一难题.

摘要： 疼痛及其治疗是临床上的一大难题,主要由于机制不明.Cdk5是一种特殊的细胞周期素依赖性激酶家族,几乎存在于整个中枢和外周神经系统的神经元内.Cdk5作为丝氨酸/苏氨酸激酶,可调节众多底物和蛋白,目前发现在疼痛信号通路及阿片耐受中具有重要作用,可能作为治疗疼痛的新方法,对其在疼痛通路及阿片耐受中作用的深入了解,将有助于解决这一难题.

摘要： 疼痛及其治疗是临床上的一大难题,主要由于机制不明.Cdk5是一种特殊的细胞周期素依赖性激酶家族,几乎存在于整个中枢和外周神经系统的神经元内.Cdk5作为丝氨酸/苏氨酸激酶,可调节众多底物和蛋白,目前发现在疼痛信号通路及阿片耐受中具有重要作用,可能作为治疗疼痛的新方法,对其在疼痛通路及阿片耐受中作用的深入了解,将有助于解决这一难题.

摘要： 疼痛及其治疗是临床上的一大难题,主要由于机制不明.Cdk5是一种特殊的细胞周期素依赖性激酶家族,几乎存在于整个中枢和外周神经系统的神经元内.Cdk5作为丝氨酸/苏氨酸激酶,可调节众多底物和蛋白,目前发现在疼痛信号通路及阿片耐受中具有重要作用,可能作为治疗疼痛的新方法,对其在疼痛通路及阿片耐受中作用的深入了解,将有助于解决这一难题.

摘要： 本申请提供式(I)的双官能化合物(I)或靶向性配体或其药学上可接受的盐、水合物、溶剂合物、前药、立体异构体或互变异构体，其作为细胞周期蛋白依赖性激酶4(CDK4)和/或细胞周期蛋白依赖性激酶6(CDK6)的蛋白降解诱导部分。本申请还涉及通过使用双官能化合物靶向降解CDK4和/或CDK6的方法，所述双官能化合物将泛素连接酶结合部分与能够结合于CDK4和/或CDK6的配体连接，能够用于治疗由CDK4和/或CDK6调节的病症。

摘要： 本申请提供式(Ia)或(Ib)的双功能化合物或其药学上可接受的盐、水合物、溶剂合物、前药、立体异构体或互变异构体，其作为细胞周期蛋白‑依赖性激酶8(CDK8)的蛋白降解诱导部分起作用。本申请还涉及通过使用双功能化合物来靶向降解CDK8的方法，所述双功能化合物将泛素连接酶‑结合部分与能够结合CDK8的配体连接，其可用于治疗由CDK8调节的疾病。

摘要： 本发明涉及抑制细胞周期蛋白依赖性激酶抑制剂(CDKI)途径的化合物和方法。更具体地讲，本发明涉及抑制CDKI途径以研究并干预老年化相关疾病和其它CDKI相关疾病的化合物和方法。本发明提供溶解度和/或效力提高的新的化合物及其使用方法。在各个方面，本发明涉及癌症的治疗。本发明提供用于化学预防和预防肿瘤复发或转移的方法。本发明还提供用于治疗某些癌症类型的诊断技术。本发明使用CDK8/19的特异性抑制剂和/或患者中CDK8水平的测量。

摘要： 本发明涉及药物化学领域，具体涉及4-(五元杂环并嘧啶/吡啶取代)氨基-1H-3-吡唑甲酰胺类衍生物、它们的制备方法、含有这些化合物的药用组合物以及它们的医疗用途，特别是作为CDK/Aurora双重抑制剂的抗肿瘤用途。

摘要： 本发明涉及靶向CDK4或CDK6的共价抑制剂及其应用，属于共价药物设计技术领域。本发明解决的技术问题是提供一种靶向CDK4或CDK6的共价抑制剂。该共价抑制剂的结构式为式I所示。本发明首次提出在Palbociclib化学结构中处于溶剂区且对活性影响不大哌嗪环上安装一个特定的共价弹头α‑氯代酰胺，与Palbociclib结合口袋的外周有一保守的氨基酸残基Thr107共价偶联，改造后的化合物并未改变原分子的母核结构，结合方式不会受到太大影响；且能够通过共价作用增加小分子与靶蛋白间的结合能力，提高抑制活性，同时降低对正常细胞的毒性。

摘要： 本发明涵盖式(I)的化合物，其中所述基团R1至R5、A和q具有权利要求和说明书中给定的含义，涉及它们作为CDK8/19抑制剂的用途、含有此类化合物的药物组合物及其作为药物尤其是作为治疗和/或预防肿瘤性疾病的药剂的用途。

摘要： 公开了作为细胞周期蛋白依赖性激酶(CDK)和细胞增殖抑制剂的其中R1是氢的式(I)的经2‑氨基嘧啶取代的2H‑吲唑化合物以及所述化合物的其中R1是在生理条件下可代谢的基团的前药，以及所述化合物和所述前药的治疗用途及制备方法。这些化合物以及其药学上可接受的盐、溶剂化物、前药、和药物组合物可用于治疗与细胞周期蛋白依赖性激酶、特别是CDK4/6的活性相关的疾病和障碍，包括但不限于各种癌症和炎症相关疾病或病症。

摘要： 本申请提供式(Ia)或(Ib)的双功能化合物或其药学上可接受的盐、水合物、溶剂合物、前药、立体异构体或互变异构体，其作为细胞周期蛋白‑依赖性激酶8(CDK8)的蛋白降解诱导部分起作用。本申请还涉及通过使用双功能化合物来靶向降解CDK8的方法，所述双功能化合物将泛素连接酶‑结合部分与能够结合CDK8的配体连接，其可用于治疗由CDK8调节的疾病。

摘要： 本申请提供式(I)的双官能化合物：

摘要： 本申请提供式(I)的双官能化合物 (I)或靶向性配体或其药学上可接受的盐、水合物、溶剂合物、前药、立体异构体或互变异构体，其作为细胞周期蛋白依赖性激酶4(CDK4)和/或细胞周期蛋白依赖性激酶6(CDK6)的蛋白降解诱导部分。本申请还涉及通过使用双官能化合物靶向降解CDK4和/或CDK6的方法，所述双官能化合物将泛素连接酶结合部分与能够结合于CDK4和/或CDK6的配体连接，能够用于治疗由CDK4和/或CDK6调节的病症。