Tanshinone ⅡA improves Alzheimer’s disease via RNA nuclearenriched abundant transcript 1/microRNA-291a-3p/member RAS oncogene family Rab22a axis

BACKGROUND Alzheimer’s disease(AD)is a neurodegenerative condition characterized by oxidative stress and neuroinflammation.Tanshinone ⅡA(Tan-ⅡA),a bioactive compound isolated from Salvia miltiorrhiza plants,has shown potential neuroprotective effects;however,the mechanisms underlying such a function remain unclear.AIM To investigate potential Tan-ⅡA neuroprotective effects in AD and to elucidate their underlying mechanisms.METHODS Hematoxylin and eosin staining was utilized to analyze structural brain tissue morphology.To assess changes in oxidative stress and neuroinflammation,we performed enzyme-linked immunosorbent assay and western blotting.Additionally,the effect of Tan-ⅡA on AD cell models was evaluated in vitro using the 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide assay.Genetic changes related to the long non-coding RNA(lncRNA)nuclear-enriched abundant transcript 1(NEAT1)/microRNA(miRNA,miR)-291a-3p/member RAS oncogene family Rab22a axis were assessed through reverse transcription quantitative polymerase chain reaction.RESULTS In vivo,Tan-ⅡA treatment improved neuronal morphology and attenuated oxidative stress and neuroinflammation in the brain tissue of AD mice.In vitro experiments showed that Tan-ⅡA dose-dependently ameliorated the amyloid-beta 1-42-induced reduction of neural stem cell viability,apoptosis,oxidative stress,and neuroinflammation.In this process,the lncRNA NEAT1-a potential therapeutic target-is highly expressed in AD mice and downregulated via Tan-ⅡA treatment.Mechanistically,NEAT1 promotes the transcription and translation of Rab22a via miR-291a-3p,which activates nuclear factor kappa-B(NF-κB)signaling,leading to activation of the pro-apoptotic B-cell lymphoma 2-associated X protein and inhibition of the anti-apoptotic B-cell lymphoma 2 protein,which exacerbates AD.Tan-ⅡA intervention effectively blocked this process by inhibiting the NEAT1/miR-291a-3p/Rab22a axis and NF-κB signaling.CONCLUSION This study demonstrates that Tan-ⅡA exerts neuroprotective effects in AD by modulating the NEAT1/miR-291a-3p/Rab22a/NF-κB signaling pathway,serving as a foundation for the development of innovative approaches for AD therapy.

The level of oncogene H-Ras correlates with tumorigenicity and malignancy

Normal bovine adrenocortical cells and some human fibroblasts can be transformed by SV40T and H-Ras in a Ras-dependent manner. We recently reported that high levels of Ras derived from 5' LTR of retrovirrus can induce highly malignant and fast growing tumors, while lower levels of Ras derived from internal ribosome entry site(IRES) promotes slower tumor growth and loss of malignancy. Ras derived from CMV promoters resulted in much lower Ras levels and loss of tumor malignancy and growth. Further studies showed that the tumors formed in the presence of lower levels of Ras and dominant negative P53(P53DD) had fewer apoptotic cells and grew faster than the tumors formed from cells with same level Ras and SV40T. Our studies suggest that low levels of Ras are insufficient to inhibit apoptosis induced by pRb inactivation. In contrast, high levels of Ras not only allow normal cells to exit senescence and form tumors, but also protect against pRb inhibition-induced cell apoptosis.

C-Ha-ras Oncogene in Oral Leukoplakia Tissues

The amplification and the G-T mutation at codon 12 of the C-Ha-ras oncogene in oral leukoplakia tissues were analyzed by using polymerase chain reaction (PCR) and molecular biologic technique. The results showed that these tissues had no amplification of Ha-ras oncogene. Only one case harbored G-T mutation in 11 oral leukoplakias, but this mutation was absent in 10 normal oral mucosal tissues. The possible role and significance of C-Ha-ras oncogene in oral precancerous lesions were also discussed.

EFFECTS OF LIMONENE,SALVIA MILTIORRHIZA AND TURMERIC DERIVATIVES ON H-RAS ONCOGENE EXPRESSION AND GAP JUNCTION INTERCELLULAR COMMUNICATION IN HUMAN SOLID TUMOR CELL LINES

Objective: To study gap junction intercellular communication (GJIC), H ras oncogene expression and ras oncogene product (P 21 ras protein) expression in four human solid tumor cell lines, W1-38,CACO 2,A549 and PaCa, and the effects of four compounds, Salvia miltiorrhiza derivative (SMD), d Limonene, Turmeric derivative I (TD I) and Turmeric derivative II (TD II), on them. Methods: The abilities of the four solid tumor cell lines to transfer dye to adjacent cells were examined by the scrape loading/dye transfer technique, and the H ras oncogene expression by Northern blotting and P 21 ras protein expression by Western blotting. Results: The results showed the loss of intercellular coupling in PaCa cells, slight GJIC in A549 and CACO 2 cells, and a good GJIC in W1-38 cells. The four compounds could improve the GJIC of PaCa to different extents. The amount of total and membrane associated P 21 ras in PaCa cells were decreased after treatment with SMD, d Limonene and TD I (2.5 μg/ml) for 48 h. Concomitantly, the growth of PaCa cells decreased in soft agar and had enhanced GJIC. The relative potency was found to be:d Limonene>SMD >TD I=TD II. There was no significant effect of the four compounds on H ras oncogene expression. Conclusion: It was suggested that there was an excellent correlation between loss of Lucifer Yellow dye transfer and ras gene mutation rate in the four solid tumor cell lines (ras gene mutation rate inversely correlated with average cell number coupled, r=0.98) i.e., the high ras gene mutation was closely correlated with loss of GJIC in these malignant human tumor cells; The antitumor effect of the monoterpene d Limonene and the phenol compound, SMD, might be related to inhibition of P 21 ras membrane association and enhancement of GJIC, whilst that of the others may be by a different mechanism; The inhibition of P 21 ras membrane association was directly related to the enhancement of gap junction intercellular com munication.

Vascular endothelial growth factor,p53,and the H-ras oncogene in Egyptian patients with bladder cancer

AIM:To evaluate the relationship between vascular endothelial growth factor(VEGF),p53,and the H-ras oncogene and different clinicopathological parameters in Egyptian patients with Schistosoma-associated transitional cell carcinoma of the bladder.METHODS:The study included 50 patients with transitional cell carcinoma for whom radical cystectomy and urinary diversions were carried out.VEGF and p53 protein expressions were evaluated with an immunohistochemical staining method,and H-ras oncogene mutations were analyzed with a polymerase chain reaction-restriction fragment length polymorphism(PCR-RFLP) technique.RESULTS:High grade tumors revealed higher p53 immunostaining than low grade tumors(P = 0.016).p53 and VEGF protein expressions,as well as H-ras oncogene mutations,had an insignificant impact on patient outcomes(P = 0.962,P = 0.791,and P = 967,respectively).Cancer extension to regional lymph nodes was associated with poor outcomes(P = 0.008).CONCLUSION:VEGF,p53 and the H-ras oncogene have no relation to patient survival and outcome in Schistosoma-associated transitional cell carcinoma.

Preliminary Study on c-Ha-ras Oncogene Mutations in Hydatidiform Mole Tissues

ve To study the presence of c-Ha-ras oncogene mutations in hydatidiform mole (HM) tissues and to further explore its relationship with mole's malignancy

子宫内膜息肉与子宫内膜癌中Ki-ras基因表达及临床意义

目的 探讨 Ki- ras基因激活与子宫内膜癌中的发生发展关系及子宫内膜息肉与子宫内膜癌的关系。方法 对子宫内膜癌及癌前病变组织进行 Ki- ras蛋白免疫组化测定 ,并利用 PCR技术检测 Ki- ras基因第一外显子 1 2密码子突变。结果 Ki- ras蛋白广泛存在于子宫内膜癌和癌前病变组织中 ,癌前病变 Ki- ras表达为 1 1 .9% ,癌组为 62 .96% ,P<0 .0 5。Ki- ras表达与细胞恶性程度呈正相关。 PCR- RFLP检测与免疫组化结果类似。结论 1 .Ki- ras基因激活可导致细胞周期增殖失控 ,是内膜癌发生发展的一个重要环节 ;2 .动态观测子宫内膜息肉中的 p2 1 ras表达阳性者 ,对子宫内膜癌的早期发现可能有积极意义。

检测胃黏膜上皮细胞微量元素、DNA、P_(53)、Ki-67、C-erbB_2、P21^(ras)研究中医脾虚证和胃癌前病变的关系

目的:探索中医脾虚证的病理生理学变化与胃黏膜癌前病变的关系。方法:对160例脾虚证胃黏膜均伴有肠上皮化生(intestinal metaplasia,IM)和/或低级别上皮内瘤变(low grade intraepithe1ial neoplasia,L-IN)患者,脾虚证分为脾气虚证(spleen Qi deficiency,SQD)、脾阴虚证(spleen Yin deficiency,SyinD)和脾虚气滞证(spleen deficiency with Qi stagnation,SDQS)三型和22例健康对照者为研究对象,采用现代科学仪器和技术检测胃黏膜上皮细胞核和线粒体的微量元素、DNA与胃黏膜P_(53),Ki-67,C-erbB_2,P21^(ras)。结果:SDQS组与L-IN间在分子生物学上也无显著性的差异。结论:要定期随访检测以上指标。有利于早期发现慢性胃炎的癌变。

子宫内膜息肉与子宫内膜癌中Ki-ras基因表达及临床意义

目的:探讨Ki-ras基因激活与子宫内膜癌中的发生发展关系及子宫内膜息肉与子宫内膜癌的关系。方法:对子宫内膜癌及癌前病变组织进行Ki-ras蛋白免疫组化测定。结果:Ki-ras蛋白广泛存在于子宫内膜癌和癌前病变组织中,癌前病变Ki-ras表达为11.9％,癌组为62.96％,P<0.05;。Ki-ras表达与细胞恶性程度呈正相关。结论:①Ki-ras基因激活可导致细胞周期增殖失控,是内膜癌发生发展的一个重要环节;②动态观测子宫内膜息肉中的P21^(ras)表达阳性者,对子宫内膜癌的早期发现可能有积极意义。

P53、P21^(ras)、Ki-67蛋白的表达及微血管密度与甲状腺癌转移关系的研究

目的探讨甲状腺癌中P53、P21ras、Ki-67基因的表达及微血管密度(MVD)与甲状腺癌转移的关系。方法用免疫组化SP法,检测45例甲状腺癌中P53、P21ras、Ki-67及血管标记物CD34蛋白的表达情况,并分析其与临床病理因素的关系。结果45例甲状腺癌中P53和P21ras的阳性表达率分别为22.2%和35.5%,差异无统计学意义;在发生淋巴结转移的13例甲状腺癌中P53蛋白阳性表达率为46.2%,明显高于无转移者的12.5%(χ2=5.77,P<0.05),其Ki-67分级指数有9例分布在Ⅱ~Ⅲ级;在复发病例中P53蛋白的阳性表达率为75%,明显高于未复发病例的10%(χ2=5.92,P<0.05),复发病例的Ki-67分级指数均在Ⅱ级。微血管密度计数在滤泡癌中为79.1±18.4,明显高于乳头状癌的35.4±12.1(t=2.412,P<0.05)。结论P53蛋白阳性表达的甲状腺癌患者易发生淋巴结转移及复发,P21ras及Ki-67的高表达则提示甲状腺癌可能发生淋巴结转移,甲状腺癌组织中的微血管密度与癌组织学类型有关,而与淋巴结转移无关。

免疫荧光双标对肝细胞癌及癌旁异型增生肝细胞Ki-67与AMACR和RAS表达的定位分析

目的对肝细胞癌(hepato celluar carcinoma,HCC)及其癌旁异型增生肝细胞Ki-67与α-甲酰基-辅酶A消旋酶(alpha-methylacyl-coenzyme A racemase,AMACR)和RAS表达进行定位分析,探讨AMACR的表达在HCC发生中的意义。方法 90例人HCC、90例癌旁肝组织制作组织芯片,以20例正常肝组织对照。用免疫荧光双标法,通过激光共聚焦显微镜,分析AMACR在肝细胞癌和癌旁异型增生肝细胞的表达与Ki-67、癌基因蛋白RAS表达的原位定位关系。结果 HCC组织中AMACR的表达显著高于癌旁肝组织,而且在HCC组织中AMACR的表达多呈弥漫性分布;HCC组织中显示Ki-67标记指数比癌旁组织高。结论 AMACR可能参与RAS信号在肝细胞异型增生和HCC早期发生的信号机制。

Targeting the“undruggable”cancer driver genes:Ras,myc,and tp53

The term“undruggable”is to describe molecules that are not targetable or at least hard to target pharmacologically.Unfortunately,some targets with potent oncogenic activity fall into this category,and currently little is known about how to solve this problem,which largely hampered drug research on human cancers.Ras,as one of the most common oncogenes,was previously considered“undruggable”,but in recent years,a few small molecules like Sotorasib(AMG-510)have emerged and proved their targeted anti-cancer effects.Further,myc,as one of the most studied oncogenes,and tp53,being the most common tumor suppressor genes,are both considered“undruggable”.Many attempts have been made to target these“undruggable”targets,but little progress has been made yet.This article summarizes the current progress of direct and indirect targeting approaches for ras,myc,two oncogenes,and tp53,a tumor suppressor gene.These are potential therapeutic targets but are considered“undruggable”.We conclude with some emerging research approaches like proteolysis targeting chimeras(PROTACs),cancer vaccines,and artificial intelligence(AI)-based drug discovery,which might provide new cues for cancer intervention.Therefore,this review sets out to clarify the current status of targeted anti-cancer drug research,and the insights gained from this review may be of assistance to learn from experience and find new ideas in developing new chemicals that directly target such“undruggable”molecules.

胰腺癌组织中p21ras蛋白表达与微血管密度的关系及其临床意义

目的检测胰腺癌组织中p21ras蛋白的表达及微血管密度(MVD)计数,探讨两者的关系及其临床意义。方法选择病理证实为胰腺导管腺癌的48例患者的石蜡切块标本,应用EnVision显色系统免疫组织化学方法进行p21ras蛋白检测和MVD计数。结果p21ras蛋白表达率胰腺癌组织为60·41%,癌旁组织为37·5%(P<0·05)。MVD计数p21ras表达阳性组为22·207±5·815,p21ras阴性组为18·053±5·502(t=3·597,P<0·01)。结论胰腺癌组织中p21ras的表达与MVD计数相关,提示ras基因突变可能促进肿瘤微血管的形成。

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。

癌性胸腔积液K-ras基因突变检测及临床应用

目的：探讨Ｋ－ｒａｓ 基因突变检测用于癌性胸腔积液的诊断价值。方法：采用ＰＣＲ－ ＳＳＣＰ技术对５８ 例癌性及３０ 例结核性胸腔积液进行Ｋ－ｒａｓ 基因突变分析。结果：结核性胸液未发现突变，癌性胸液有１７ 例突变阳性，突变率２９－３ ％ ，其中腺癌所致胸腔积液突变率为３４－１％ （１４／２１），鳞癌１６－７ ％（２／１２）。１７ 例Ｋ－ｒａｓ 基因突变阳性的胸液中，１４ 例为肉眼血性，明显高于非血性胸液组，Ｐ＜ ０－０５。１８ 例未找到原发病灶的胸液中４４－４％ Ｋ－ ｒａｓ 基因突变阳性。４９ 例患者随访１０ 个月，Ｋ－ｒａｓ 基因突变阳性者死亡率高达８０－０ ％ ，而无Ｋ－ｒａｓ 基因突变者死亡率明显降低，为２６－５ ％ ，Ｐ＜ ０－０５ 。结论：Ｋ－ｒａｓ 基因突变检测是诊断癌性胸腔积液的又一有效手段，在某些情况下显示出特有的优势，并且对预后的判断有一定价值。

胰腺癌ras癌基因及p53抑癌基因表达的临床意义

目的研究ras癌基因及p53抑癌基因在在胰腺癌表达的临床意义．方法胰腺石蜡包埋标本55例，包括胰腺癌32例，癌切缘未受浸润的胰腺组织12例，急慢性胰腺炎7例，正常胰腺4例，标本均经病理学证实，用免疫组织化学ABC法对上述标本的ras癌基因及p53抑癌基因表达进行检测．结果在32例胰腺癌中，ras和p53基因的阳性表达率分别为71．9％和28．1％，高于胰腺炎和癌切缘组织（P＜0．05）ras，p53基因表达与患者性别、年龄、肿瘤所在部位及大小和初发症状无关（P＞0．05），p53基因表达与临床分期和病理分级相关（P＜0．05），p53基因表达阳性者其临床分期较晚期，细胞分化较差，而ras基因表达仅与病理分级有关（P＜0．05）．P53基因表达与癌肿可切除率相关（P＜0．05），凡癌肿能切除者多为p53基因表达阴性者.p53基因表达亦与淋巴结转移有关（P＜0．05），其表达阳性者多已有淋巴结转移．ras与p53基因表达之间存在正相关关系．结论ras与p53基因表达可以反映胰腺癌的生物学行为，对胰腺癌的诊断和治疗有一定指导意义．

粪便中检测K-ras基因突变对老年大肠癌诊断价值的研究

探讨粪便K ras基因检测在老年大肠癌临床诊断中的价值。收集连续就诊的 2 3例老年大肠癌患者、2 0例结肠腺瘤性息肉患者及 2 0名健康老年查体者的粪便 ,并从中提取DNA ,应用等位基因特异性杂交技术检测粪便K ras基因第 12位密码子第 1、2位碱基突变情况。结果K ras基因突变率在大肠癌患者为 5 6 5 2 % (13/ 2 3) ,明显高于正常查体者的 5 % (1/ 2 0 ) (P <0 0 1) ,与结肠腺瘤性息肉组的 30 % (6 / 2 0 )比较 ,差异无显著性意义 (P >0 0 5 )。 92 31% (12 / 13)的大肠癌K ras基因突变位点发生在第 12位密码子第 2位碱基。研究表明 ,结肠癌患者组织及粪便中K ras基因突变的检出具有良好的一致性 ,提示粪便中检测K

乳腺不典型增生组织中ras基因产物表达的意义

用免疫组化法检测正常乳腺组织、乳腺囊性增生病和乳腺癌中ｒａｓ癌基因产物ｐ２１蛋白表达。结果显示正常乳腺组织无ｐ２１蛋白表达，乳腺囊性增生病不典型增生Ⅰ、Ⅱ、Ⅲ级，乳腺癌组织分化Ⅰ、Ⅱ、Ⅲ级ｐ２１蛋白表达阳性率分别为１０％、３０％、４０％、４６％、６４％和８４％。乳腺癌不同组织学类型中ｐ２１蛋白表达阳性率差别无显著性。在乳腺癌前的不典型增生阶段已有ｒａｓ癌基因产物的过度表达，随着不典型增生程度加重其表达阳性率增加，提示ｒａｓ癌基因改变及其产物表达增多可发生在乳腺上皮细胞癌变之前和其进展期，与乳腺癌发生及其生物学行为密切相关。可能成为临床监测乳腺癌前病变的一种有重要价值的参考指标。

RASA1在胰腺癌中的异常表达及其临床意义

目的:探讨Ras p21蛋白活化子1(Ras p21 protein activator 1,RASA1)在胰腺癌中的表达状况及可能作用。方法:以qRT-PCR检测胰腺癌细胞(Capan-2、CFPAC-1、BxPC-3)和胰腺导管上皮细胞(H6C7)中RASA1 mRNA表达水平的差异,以Western blotting检测上述细胞之间RASA1蛋白表达水平的差异;以免疫组化检测RASA1蛋白在胰腺癌及胰腺良性病变(慢性胰腺炎、胰腺囊肿)中的表达差异,并观察其表达水平与胰腺癌各临床病理因素之间的联系。结果:各胰腺癌细胞株中RASA1 mRNA和蛋白表达水平均低于胰腺导管上皮细胞(P<0.05)。肿瘤组织RASA1蛋白表达水平显著低于良性病变组织(P<0.05);侵犯周边器官的肿瘤组织中RASA1表达显著低于局限于胰腺内的组织(P<0.05);Ⅰ期胰腺癌组织RASA1的表达则显著高于Ⅱ、Ⅲ期的癌组织(P<0.05);但RASA1表达与胰腺癌的远处转移关系尚不明确。结论:RASA1作为抑癌蛋白可能在胰腺癌的发生发展中发挥重要作用。

d-宁烯、丹参及姜黄素衍生物对ras基因产物膜结合和细胞间隙信息传导的影响

目的旨在寻找新型抗肿瘤药物，进一步研究ｄ宁烯、丹参及姜黄素衍生物的抗肿瘤机理。采用分子生物学方法及划痕标记染料示踪技术，研究了４种人实体瘤起源的细胞系的细胞间隙信息传导（ＧＪＩＣ）、Ｈｒａｓ癌基因表达以及ｒａｓ癌基因产物（Ｐ２１ｒａｓ蛋白）表达状态，并观察了４种天然产物对它们的影响。结果表明，细胞内染料传输功能的丧失与ｒａｓ基因突变率呈正相关；单萜化合物ｄ宁烯和酚类化合物丹参衍生物的抗肿瘤作用可能与抑制Ｐ２１ｒａｓ蛋白膜结合和增强细胞间隙信息传导功能有关。