二氯化镭223对去势抵抗性前列腺癌伴骨转移患者血细胞计数骨痛程度和血PSA f-PSA和OPG的影响

目的:探究二氯化镭223对去势抵抗性前列腺癌(CRPC)伴骨转移患者血细胞计数、骨痛程度和血前列腺特异性抗原(PSA)、游离PSA(f-PSA)和骨保护素(OPG)的影响。方法:研究西安交通大学第一附属医院2020年2月至2023年12月收治的122例CRPC伴骨转移患者,采用随机数字法将上述患者分为观察组(n=61,采用二氯化镭223+常规治疗)和对照组(n=61,采用常规治疗),6个月后,比较两组患者血细胞计数、骨痛程度、血清因子、疗效、不良反应。结果:治疗后,两组红细胞、NK细胞、CD4+、血小板计数均有下降,治疗前后差值具有统计学意义(P<0.05);治疗后,两组VAS、PSA、f-PSA、OPG均有下降,治疗前后差值具有统计学意义(P<0.05)。观察组总有效率高于对照组(P<0.05);观察组胃肠道不适、肌肉酸痛或乏力、体温异常、周围性水肿单项不良反应发生率及合计发生率(6.56%、13.11%、9.84%、11.48%、40.98%)与对照组(8.20%、9.84%、11.48%、3.28%、32.79%)比较时,差异均无统计学意义(P>0.05)。结论:对于CRPC伴骨转移患者而言,二氯化镭223有利于改善其血细胞计数及OPG水平,减轻骨痛严重程度,降低PSA和f-PSA水平,增强疗效,且安全性较高,具有推广价值。

反刍动物初乳microRNA组成和功能研究进展

反刍动物初乳中含有丰富的生物活性成分,其中microRNA是一类非编码RNA,可在转录后水平调节基因的表达,对于母体乳腺以及幼龄反刍动物肠道发育具有重要的调控作用。近年来,反刍动物初乳microRNA组成和功能的研究开始受到关注,本文综述了反刍动物初乳中microRNA的来源、组成及其影响因素、功能,以及目前研究的局限性和未来的研究方向,为生产高品质初乳,提高母仔一体化培育水平提供理论支撑。

携载microRNA-140外泌体/海藻酸钠/胶原水凝胶修复关节软骨损伤

背景:研究已证实,上调microRNA-140表达可部分抑制膝关节软骨组织与细胞的骨关节炎样改变,延缓骨关节炎进程,提示microRNA-140参与了骨关节炎的发病机制。目的:采用海藻酸钠/胶原水凝胶负载过表达microRNA-140的外泌体,进一步分析microRNA-140参与骨关节炎的相关机制。方法:利用慢病毒感染大鼠骨髓间充质干细胞使其过表达microRNA-140,随后分离提取外泌体,得到过表达microRNA-140的外泌体。制备负载外泌体的海藻酸钠/胶原水凝胶。采用随机数字表法将32只SD大鼠随机分为4组,每组8只:正常对照组不进行任何处理,骨关节炎组、未转染外泌体组、转染外泌体组均通过膝关节腔内注射碘乙酸钠的方式建立骨关节炎模型,造模2周后,骨关节炎组膝关节腔内注射PBS,未转染外泌体组、转染外泌体组膝关节腔内分别注射负载未过表达microRNA-140与过表达microRNA-140外泌体的海藻酸钠/胶原水凝胶。造模后第6周,检测大鼠机械刺激缩足反应阈值、滑膜液炎症因子浓度、软骨相关基因表达、膝关节软骨组织的组织学变化与焦亡相关蛋白表达。结果与结论:①与正常对照组比较,骨关节炎组机械刺激缩足反应阈值、Ⅱ型胶原及SOX9 mRNA表达、Ⅱ型胶原免疫荧光强度均减少(P<0.05),滑膜液中促炎症因子水平增加(P<0.05),基质金属蛋白酶13、血小板反应蛋白解整合素金属肽酶5(ADAMTS5)mRNA表达增加(P<0.05),NLRP3、ASC、GSDMD p30、caspase-1 p20、白细胞介素1β、白细胞介素18蛋白表达均增加(P<0.05),GSDMD、cleaved caspase-1免疫荧光强度增强(P<0.05),软骨组织损伤严重。②与骨关节炎组比较,两外泌体组机械刺激缩足反应阈值、Ⅱ型胶原及SOX9 mRNA表达、Ⅱ型胶原免疫荧光强度均增加(P<0.05),滑膜液中促炎症因子水平减少(P<0.05),基质金属蛋白酶13 mRNA表达减少(P<0.05),NLRP3、ASC、GSDMD p30、caspase-1 p20、白细胞介素1β、白细胞介素18的蛋白表达均减少(P<0.05),GSDMD、cleaved caspase-1的免疫荧光强度减弱(P<0.05),软骨组织损伤减轻(P<0.05),并且转染外泌体组的作用更强。③结果表明,microRNA-140可通过抑制炎症、维持软骨稳态、抑制软骨焦亡来减轻骨关节炎大鼠的疼痛反应,降低软骨损伤,发挥骨关节炎治疗作用。

Acquired sensorineural hearing loss,oxidative stress,and microRNAs

Hearing loss is the third leading cause of human disability.Age-related hearing loss,one type of acquired sensorineural hearing loss,is largely responsible for this escalating global health burden.Noise-induced,ototoxic,and idiopathic sudden sensorineural are other less common types of acquired hearing loss.The etiology of these conditions is complex and multi-fa ctorial involving an interplay of genetic and environmental factors.Oxidative stress has recently been proposed as a likely linking cause in most types of acquired sensorineural hearing loss.Short non-coding RNA sequences known as microRNAs(miRNAs)have increasingly been shown to play a role in cellular hypoxia and oxidative stress responses including promoting an apoptotic response.Sensory hair cell death is a central histopathological finding in sensorineural hearing loss.As these cells do not regenerate in humans,it underlies the irreversibility of human age-related hearing loss.Ovid EMBASE,Ovid MEDLINE,Web of Science Core Collection,and ClinicalTrials.gov databases over the period August 1,2018 to July 31,2023 were searched with"hearing loss,""hypoxamiRs,""hypoxia,""microRNAs,""ischemia,"and"oxidative stress"text words for English language primary study publications or registered clinical trials.Registe red clinical trials known to the senior author we re also assessed.A total of 222studies were thus identified.After excluding duplicates,editorials,retra ctions,secondary research studies,and non-English language articles,39 primary studies and clinical trials underwent full-text screening.This resulted in 11 animal,in vitro,and/or human subject journal articles and 8 registered clinical trial database entries which form the basis of this narrative review.MiRNAs miR-34a and miR-29b levels increase with age in mice.These miRNAs were demonstrated in human neuroblastoma and murine cochlear cell lines to target Sirtuin 1/peroxisome proliferato r-activated receptor gamma coactivator-1-alpha(SIRT1/P GC-1α),SIRT1p53,and SIRT1/hypoxia-inducible factor 1-alpha signaling pathways resulting in increased apoptosis.Furthermore,hypoxia and oxidative stress had a similar adve rse apoptotic effect,which was inhibited by resve ratrol and a myocardial inhibitorassociated transcript,a miR-29b competing endogenous mRNA.Gentamicin reduced miR-182-5p levels and increased cochlear oxidative stress and cell death in mice-an effect that was corrected by inner ear stem cell-derived exosomes.There is ongoing work seeking to determine if these findings can be effectively translated to humans.

MicroRNAs as potential biomarkers for diagnosis of post-traumatic stress disorder

Post-traumatic stress disorder is a mental disorder caused by exposure to severe traumatic life events.Currently,there are no validated biomarkers or laboratory tests that can distinguish between trauma survivors with and without post-traumatic stress disorder.In addition,the heterogeneity of clinical presentations of post-traumatic stress disorder and the overlap of symptoms with other conditions can lead to misdiagnosis and inappropriate treatment.Evidence suggests that this condition is a multisystem disorder that affects many biological systems,raising the possibility that peripheral markers of disease may be used to diagnose post-traumatic stress disorder.We performed a PubMed search for microRNAs(miRNAs)in post-traumatic stress disorder(PTSD)that could serve as diagnostic biomarkers and found 18 original research articles on studies performed with human patients and published January 2012 to December 2023.These included four studies with whole blood,seven with peripheral blood mononuclear cells,four with plasma extracellular vesicles/exosomes,and one with serum exosomes.One of these studies had also used whole plasma.Two studies were excluded as they did not involve microRNA biomarkers.Most of the studies had collected samples from adult male Veterans who had returned from deployment and been exposed to combat,and only two were from recently traumatized adult subjects.In measuring miRNA expression levels,many of the studies had used microarray miRNA analysis,miRNA Seq analysis,or NanoString panels.Only six studies had used real time polymerase chain reaction assay to determine/validate miRNA expression in PTSD subjects compared to controls.The miRNAs that were found/validated in these studies may be considered as potential candidate biomarkers for PTSD and include miR-3130-5p in whole blood;miR-193a-5p,-7113-5p,-125a,-181c,and-671-5p in peripheral blood mononuclear cells;miR-10b-5p,-203a-3p,-4488,-502-3p,-874-3p,-5100,and-7641 in plasma extracellular vesicles/exosomes;and miR-18a-3p and-7-1-5p in blood plasma.Several important limitations identified in the studies need to be taken into account in future studies.Further studies are warranted with war veterans and recently traumatized children,adolescents,and adults having PTSD and use of animal models subjected to various stressors and the effects of suppressing or overexpressing specific microRNAs.

Autism spectrum disorder:difficulties in diagnosis and microRNA biomarkers

We performed a PubMed search for microRNAs in autism spectrum disorder that could serve as diagnostic biomarkers in patients and selected 17 articles published from January 2008 to December 2023,of which 4 studies were performed with whole blood,4 with blood plasma,5 with blood serum,1 with serum neural cell adhesion molecule L1-captured extracellular vesicles,1 with blood cells,and 2 with peripheral blood mononuclear cells.Most of the studies involved children and the study cohorts were largely males.Many of the studies had performed microRNA sequencing or quantitative polymerase chain reaction assays to measure microRNA expression.Only five studies had used real-time polymerase chain reaction assay to validate microRNA expression in autism spectrum disorder subjects compared to controls.The microRNAs that were validated in these studies may be considered as potential candidate biomarkers for autism spectrum disorder and include miR-500a-5p,-197-5p,-424-5p,-664a-3p,-365a-3p,-619-5p,-664a-3p,-3135a,-328-3p,and-500a-5p in blood plasma and miR-151a-3p,-181b-5p,-320a,-328,-433,-489,-572,-663a,-101-3p,-106b-5p,-19b-3p,-195-5p,and-130a-3p in blood serum of children,and miR-15b-5p and-6126 in whole blood of adults.Several important limitations were identified in the studies reviewed,and need to be taken into account in future studies.Further studies are warranted with children and adults having different levels of autism spectrum disorder severity and consideration should be given to using animal models of autism spectrum disorder to investigate the effects of suppressing or overexpressing specific microRNAs as a novel therapy.

Diagnostic utility of microRNA profiles in cavitatory and noncavitatory pulmonary tuberculosis:Research protocol

BACKGROUND Tuberculosis(TB)is a common infection causing huge morbidity and mortality to mankind.The analytical methods used in diagnosing TB are not sensitive in paucibacillary infections and also require trained technical personnel.MicroRNAs are stable in serum and other body fluids,and hold great potential in the diagnosis of TB.AIM To analyze the dysregulated microRNA profiles among patients with cavitatory and non-cavitatory pulmonary TB.METHODS The prospective study will be conducted in a tertiary care center in India.Adult patients with newly diagnosed pulmonary TB will be included.There will be two groups:Patients with sputum positive pulmonary TB with cavity and without cavity(group1),and apparently healthy individuals(group 2).The participants will undergo sputum examination,Xpert Mycobacterium TB complex/resistance to rifampin(Mtb/RIF)assay,chest X-ray,and blood investigations and serum microRNA detection.Ethics approval has been obtained.Written informed consent will be obtained.Appropriate statistical analyses will be used.RESULTS MicroRNAs will be correlated with sputum positivity,Xpert Mtb/RIF assay,radiological involvement,inflammatory markers,and course of the disease among cases and controls.CONCLUSION MicroRNAs could serve as potential diagnostic biomarkers in diagnostically challenging TB patients.

MicroRNAs as potential diagnostic biomarkers for bipolar disorder

Abnormal expression of microRNAs is connected to brain development and disease and could provide novel biomarkers for the diagnosis and prognosis of bipolar disorder. We performed a PubMed search for microRNA biomarkers in bipolar disorder and found 18 original research articles on studies performed with human patients and published from January 2011 to June 2023. These studies included microRNA profiling in bloodand brain-based materials. From the studies that had validated the preliminary findings,potential candidate biomarkers for bipolar disorder in adults could be miR-140-3p,-30d-5p,-330-5p,-378a-5p,-21-3p,-330-3p,-345-5p in whole blood, miR-19b-3p,-1180-3p,-125a-5p, let-7e-5p in blood plasma, and miR-7-5p,-23b-5p,-142-3p,-221-5p,-370-3p in the blood serum. Two of the studies had investigated the changes in microRNA expression of patients with bipolar disorder receiving treatment. One showed a significant increase in plasma miR-134 compared to baseline after 4 weeks of treatment which included typical antipsychotics, atypical antipsychotics, and benzodiazepines. The other study had assessed the effects of prescribed medications which included neurotransmitter receptorsite binders(drug class B) and sedatives, hypnotics, anticonvulsants, and analgesics(drug class C) on microRNA results. The combined effects of the two drug classes increased the significance of the results for miR-219 and-29c with miR-30e-3p and-526b* acquiring significance. MicroRNAs were tested to see if they could serve as biomarkers of bipolar disorder at different clinical states of mania, depression, and euthymia. One study showed that upregulation in whole blood of miR-9-5p,-29a-3p,-106a-5p,-106b-5p,-107,-125a-3p,-125b-5p and of miR-107,-125a-3p occurred in manic and euthymic patients compared to controls, respectively, and that upregulation of miR-106a-5p,-107 was found for manic compared to euthymic patients. In two other studies using blood plasma,downregulation of miR-134 was observed in manic patients compared to controls, and dysregulation of miR-134,-152,-607,-633,-652,-155 occurred in euthymic patients compared to controls. Finally, microRNAs such as miR-34a,-34b,-34c,-137, and-140-3p,-21-3p,-30d-5p,-330-5p,-378a-5p,-134,-19b-3p were shown to have diagnostic potential in distinguishing bipolar disorder patients from schizophrenia or major depressive disorder patients, respectively. Further studies are warranted with adolescents and young adults having bipolar disorder and consideration should be given to using animal models of the disorder to investigate the effects of suppressing or overexpressing specific microRNAs.

Extracellular matrix gene set and microRNA network in intestinal ischemia-reperfusion injury:Insights from RNA sequencing for diagnosis and therapy

Intestinal ischemia-reperfusion injury(IIRI)is a complex and severe pathophysiological process characterized by oxidative stress,inflammation,and apoptosis.In recent years,the critical roles of extracellular matrix(ECM)genes and microRNAs(miRNAs)in IIRI have garnered widespread attention.This review aims to systematically summarize the diagnostic and therapeutic potential of ECM gene sets and miRNA regulatory networks in IIRI.First,we review the molecular mechanisms of IIRI,focusing on the dual role of the ECM in tissue injury and repair processes.The expression changes and functions of ECM components such as collagen,elastin,and matrix metalloproteinases during IIRI progression are deeply analyzed.Second,we systematically summarize the regulatory roles of miRNAs in IIRI,particularly the mechanisms and functions of miRNAs such as miR-125b and miR-200a in regulating inflammation,apoptosis,and ECM remodeling.Additionally,this review discusses potential diagnostic biomarkers and treatment strategies based on ECM genes and miRNAs.We extensively evaluate the prospects of miRNA-targeted therapy and ECM component modulation in preventing and treating IIRI,emphasizing the clinical translational potential of these emerging therapies.In conclusion,the diagnostic and therapeutic potential of ECM gene sets and miRNA regulatory networks in IIRI provides new directions for further research,necessitating additional clinical and basic studies to validate and expand these findings for improving clinical outcomes in IIRI patients.

MicroRNA-214调控骨关节炎软骨和软骨下骨代谢的机制

背景:microRNA-214(miR-214)在骨质疏松中的作用国内外已有相关报道,而miR-214与骨关节炎关节软骨及软骨下骨退变之间的相互关系尚不清楚。目的:探讨miR-214与小鼠膝骨关节炎软骨及软骨下骨退变之间存在的关系。方法:取30只C57BL/6J小鼠随机分组:①实验一:分为假手术组和内侧半月板失稳组(n=3),分别进行苏木精-伊红染色和荧光定量PCR检测miR-214基因的表达变化;②实验二:分为假手术组、内侧半月板失稳组、内侧半月板失稳+空载腺病毒组(空载组)、内侧半月板失稳+miR-214拮抗剂过表达腺病毒组(拮抗剂组)(n=6),术后4周各组分别取软骨组织,进行苏木精-伊红、番红O固绿、甲苯胺蓝染色分析;荧光定量PCR、Western blot检测关节软骨中相关因子的表达情况。结果与结论:①实验一中,苏木精-伊红染色结果显示,与假手术组相比,内侧半月板失稳组可见软骨退变;荧光定量PCR检测结果显示,所有样本均有miR-214表达,而内侧半月板失稳组软骨样本中miR-214的表达水平明显高于假手术组(P<0.05);②实验二中,苏木精-伊红染色、番红O固绿染色、甲苯胺蓝染色结果显示,拮抗剂组软骨退变程度低于内侧半月板失稳组;腺病毒验证PCR检测结果显示,空载组软骨中miR-214表达水平高于拮抗剂组(P<0.05);③实验二中,X射线片显示,内侧半月板失稳组和空载组呈典型骨关节炎影像学变化,拮抗剂组关节退行性病变程度相对较轻;Mirco-CT检测结果显示,拮抗剂组在注入miR-214拮抗剂后,骨小梁结构模型指数变小,各项数据整体好于内侧半月板失稳组及空载组;④实验二Western blot检测结果显示,内侧半月板失稳组、空载组软骨标本中软骨相关因子Ⅱ型胶原α1、性别决定区Y框转录因子9、Runt相关转录因子2、骨桥蛋白的相对表达水平低于假手术组及拮抗剂组(P<0.05);而金属基质蛋白酶13的相对表达水平在内侧半月板失稳组、空载组高于假手术组及拮抗剂组(P<0.05);⑤实验二荧光定量PCR检测结果显示,与假手术组比较,肿瘤坏死因子α和白细胞介素6 mRNA的相对表达量在内侧半月板失稳组、空载组中表达相对较高,拮抗剂组中表达相对较低(P<0.05);内侧半月板失稳组、空载组高于拮抗剂组(P<0.05);⑥结果表明,骨关节炎小鼠模型的关节软骨中miR-214表达水平明显升高,提示miR-214表达水平的升高与骨关节炎有密切联系;而在骨关节炎小鼠模型膝关节腔内注入miR-214拮抗剂,可以延缓关节软骨退化、促进软骨下骨重塑,改善骨关节炎进展。

循环microRNA-223水平与急性冠脉综合征患者的血小板反应及临床预后相关性的研究

目的研究血浆microRNA-223(miR-223)表达水平与急性冠脉综合征(ACS)患者服用氯吡格雷后血小板反应及临床预后的关系。方法连续纳入接受经皮冠状动脉介入治疗(PCI)的ACS患者208例,术前均接受负荷剂量的氯吡格雷+阿司匹林的双联抗血小板聚集治疗(DAPT)。采用实时荧光定量PCR(qPCR)检测血浆miR-223表达水平,流式细胞术检测血小板反应指数(PRI)。根据PRI中位数将患者分为低PRI组(PRI≤56.3%)和高PRI组(PRI>56.3%),各104例。比较2组患者血浆miR-223表达水平和主要临床及生化指标。随访2年,通过Cox比例风险回归分析血浆miR-223表达水平、PRI、肌钙蛋白I(TnI)、B型钠尿肽(BNP)等指标对主要不良心血管事件(MACE)的影响因素。通过受检者工作特征(ROC)曲线评价血浆miR-223、PRI对MACE的预测能力。结果miR-223表达水平与PRI呈负相关(rs=-0.420,P<0.05)。低PRI组患者血浆miR-223表达水平高于高PRI组[(1.15(0.58,1.80)vs.0.64(0.26,1.08),Z=0.471,P<0.05]。30例(14.4%)患者发生MACE,低PRI组MACE发生率低于高PRI组(P<0.05)。Cox比例风险回归分析显示,血浆miR-223和PRI是ACS患者发生MACE的独立预测因子。血浆miR-223和PRI预测ACS患者发生MACE的ROC曲线下面积分别为0.700(95%CI:0.609~0.791,P<0.05)和0.710(95%CI:0.606~0.815,P<0.05)。结论循环miR-223表达水平与ACS患者服用氯吡格雷后PRI呈负相关,循环miR-223和PRI是ACS患者PCI术后MACE的独立预测因子。

microRNA-223对糖基化终产物诱导人脂肪间充质干细胞凋亡和氧化应激影响的体外研究

目的观察microRNA-223(miR-223)对糖基化终产物(AGE)诱导人脂肪间充质干细胞(h ADSC)凋亡和氧化应激的影响。方法采用酶消化法分离培养h ADSC,并应用流式细胞术对表面抗原CD14、CD34、CD45、CD90、CD105和人类白细胞抗原DR(HLA-DR)进行检测。将h ADSC分为牛血清白蛋白(BSA)对照组、AGE修饰的牛血清白蛋白(AGE-BSA)作用组、miR-223模拟物转染组、miR-223模拟物转染+AGE-BSA组、miR-223抑制物转染组和miR-223抑制物转染+AGE-BSA组。应用CCK-8法和TUNEL染色检测各组细胞存活率和凋亡率,Western blot检测Cleaved Caspase3蛋白表达水平,应用双氯荧光素(DCFH-DA)试剂盒检测各组细胞活性氧(ROS)含量。结果流式细胞术检测结果表明,原代培养的h ADSC高表达CD14、CD90和CD105,不表达CD34、CD45和HLADR。CCK-8法、TUNEL染色、Western blot和DCFH-DA法检测结果表明,与BSA对照组相比,AGE-BSA作用组h ADSC凋亡率、miR-223表达水平、Cleaved Caspase3蛋白表达水平、ROS生成显著升高,而细胞存活率下降(P<0.05);与AGE-BSA作用组相比,miR-223模拟物转染能够进一步上调AGE-BSA引起的h ADSC凋亡率、Cleaved Caspase3蛋白表达水平和ROS生成增加,下调AGE-BSA引起的h ADSC存活率减少(P<0.05);与AGE-BSA作用组相比,miR-223抑制物转染能够抑制h ADSC凋亡率、Cleaved Caspase3蛋白表达水平和ROS生成增加,拮抗AGEBSA引起的h ADSC存活率减少(P<0.05)。结论 miR-223高表达能够促进AGE-BSA引起的h ADSC细胞凋亡和ROS生成,其可能作为调控h ADSC促进糖尿病创伤愈合的新靶点。

MicroRNA-223表达与肝癌根治性切除术预后的相关性

目的识别可以作为肝癌根治性切除术患者预后标志物的microRNA(miRNA)分子。方法利用miRNA微阵列方法对2例原发性肝癌及对应的肺转移性肝癌进行miRNA表达分析。将原发性和转移性肝癌中表达量有2倍差异的miRNAs作为候选miRNAs分子。在miRNA验证过程中,运用实时荧光定量聚合酶链反应(qRT-PCR)分析37例肝癌及相应癌旁非肿瘤组织中候选miRNAs分子的表达,并将其与患者的临床病理特征及生存情况进行相关性分析。结果最终选取8种miRNA(smiR-27b、122、142-5p、196a、223、590-5p、630及944)作为候选miRNA。只有miR-223表达水平与肿瘤分期、有丝分裂指数相关。将肝癌患者分为miR-223高表达组(25例)和miR-223低表达组(12例)后发现,miR-223高表达与较高T分期、淋巴结转移、较高丝分裂指数及较高Ki-67阳性指数相关。此外,miR-223高表达还与总体生存率和无病存活率下降相关(P<0.05),中位随访时间37.9个月[疾病复发危险比为16.267(95%CI:1.732,153.789)P=0.015]。结论肝癌组织中miR-223异常表达与肝癌患者治疗结束后发生复发转移,以及无病生存时间和总生存率有关,通过检测肿瘤组织中miR-223 qRT-PCR反应有可能预测患者预后。

microRNA⁃223在动脉粥样硬化发生过程中的网络调控机制

microRNA⁃223(miR⁃223)是参与动脉粥样硬化(atherosclerosis,AS)炎性调控、细胞生长等通路的微小非编码RNA。本研究系统地探究miR⁃223及其靶基因的网络调控机制,以便全面理解miR⁃223在AS中的作用。利用miRNA靶基因预测数据库miRDB、miRmap、TargetScan和miRTarBase获取miR⁃223的靶基因集。R语言分析基因表达综合数据库(gene expression omnibus,GEO)共享平台动脉粥样硬化斑块差异表达基因集(GSE100927),筛选出斑块差异表达基因,并与miR⁃223靶基因集交叉匹配。利用基因本体(gene ontology,GO)及基因组数据库(kyoto encyclopedia of genes and genomes,KEGG)分析研究差异表达基因功能。结果显示,斑块中下调的1584个差异表达基因与miR⁃223靶基因交叉匹配得到422个交集mRNA。GO及KEGG富集分析发现miR⁃223可能通过细胞生长、炎症反应以及血管平滑肌收缩等信号通路调节动脉粥样硬化斑块的发生发展过程。蛋白相互作用网络(protein⁃protein interaction networks,PPI)分析获得关键节点基因是INADL、JAM3、SMTN、LDB3、YAP1、TJP1、NCKAP1、PDLIM3、MICAL2和MPP5,其中YAP1也与铜死亡相关。我们还发现miR⁃223可能直接靶向GLS、GCSH调控铜死亡,参与动脉粥样硬化的发生发展过程。本研究表明,miR⁃223主要通过调控细胞生长、铜死亡等相关信号通路影响动脉粥样硬化的各个进程。

microRNA-223调控人胚胎干细胞向树突细胞分化

目的:建立人胚胎干细胞(ESC)向树突细胞诱导分化的新策略,探讨microRNA-223(miR-223)在人胚胎干细胞源树突细胞产生过程中的调控作用及其分子机制。方法:采用人胚胎干细胞在胞外基质Ⅳ型胶原蛋白上直接贴壁培养,加入造血生长因子分步向造血干/祖细胞、共同髓系祖细胞和树突细胞诱导的方案,通过形态学、流式细胞术和造血集落形成实验鉴定分化细胞;人胚胎干细胞经慢病毒转染过表达miR-223或抑制其表达后启动向树突细胞分化,比较不同miR-223表达水平下分化细胞中造血集落形成的数目和表面标记物的表达量;应用双荧光素酶报告基因检测验证TGFBR3是miR-223发挥作用的直接靶标。结果:人ES细胞成功诱导为树突细胞,分化细胞中表达CD83比例可达82%,在整个分化过程中miR-223表达呈上调趋势;添加miR-223模拟物组分化细胞表达CD34^+CD45^+、CD34^+CD45^+以及CD83^+的比例均显著高于添加miR-223抑制剂组和阴性对照组(P<0.05);添加miR-223抑制剂组分化细胞表达各阶段细胞标记物显著低于阴性对照组(P<0.05);添加miR-223模拟物组分化细胞出现大约759个CFU/105细胞数,显著高于其它各组(P<0.05);双荧光素酶报告基因结果显示,miR-223显著抑制TGFBR3-3'UTR结构的荧光素酶活性(下降了37%)(P<0.05),而且TGFBR3-3'UTR突变型的荧光素酶活性显著高于野生型(P<0.01);随着向树突细胞分化成熟,添加miR-223模拟物组分化细胞表达TGFBR3水平逐渐下降,而添加miR-223抑制剂组由于内源性miR-223受到抑制而明显上调TGFBR3的表达。结论:miR-223调控人胚胎干细胞向树突细胞分化,可能通过直接作用于靶标TGFBR3而促进胚胎干细胞源树突细胞的产生。

结肠癌组织microRNA-223、FBXW7的表达及与其临床病理参数和预后的关系

目的研究结肠癌组织中microRNA-223(miR-223)、FBXW7的表达及其与临床病理参数和预后的关系。方法收集2015年1月—2017年4月钦州市第一人民医院146例经手术切除的结肠癌组织和癌旁组织,采用实时荧光定量聚合酶链反应(qRT-PCR)检测结肠癌组织中mi R-223、FBXW7表达。通过在线网站预测miR-223与FBXW7存在结合位点。Pearson法分析两者表达的相关性及其与临床病理参数的关系。根据结肠癌组织中miR-223、FBXW7表达的均值分为miR-223高表达组与miR-223低表达组,FBXW7高表达组与FBXW7低表达组。用Kaplan-Meier法绘制不同mi R-223、FBXW7表达结肠癌患者的生存曲线。多因素Cox回归分析结肠癌患者预后的影响因素。结果结肠癌组织miR-223 m RNA相对表达量高于癌旁组织(P<0.05),FBXW7mRNA相对表达量低于癌旁组织(P<0.05)。病理分期Ⅲ期、有淋巴结转移结肠癌组织mi R-223mRNA相对表达量高于Ⅰ、Ⅱ期和无淋巴结转移(P<0.05);病理分期Ⅲ期、有淋巴结转移结肠癌组织FBXW7mRNA相对表达量低于Ⅰ、Ⅱ期和无淋巴结转移(P<0.05)。不同性别、年龄、肿瘤大小、分化程度及有无侵犯浆膜结肠癌组织miR-223、FBXW7mRNA相对表达量比较,差异无统计学意义(P>0.05)。Pearson相关系数分析显示,结肠癌组织miR-223表达与FBXW7表达呈负相关(r=-0.679,P<0.05)。术后随访8~60个月,随访期间死亡35例,总生存率为76.03%(111/146)。miR-223高表达组总生存率低于mi R-223低表达组(P<0.05)。FBXW7高表达组总生存率高于FBXW7低表达组(P<0.05)。单因素Cox回归分析结果显示,侵犯浆膜[HR=1.454(95%CI:1.086,1.947)]、病理分期Ⅲ期[HR=1.744(95%CI:1.070,2.840)]、淋巴结转移[HR=2.896(95%CI:1.114,7.531)]、miR-223≥4.76[HR=2.196(95%CI:1.085,4.445)]为结肠癌患者预后的危险因素(P<0.05),FBXW7≥1.23[HR=0.388(95%CI:0.172,0.875)]为保护因素(P<0.05)。多因素Cox回归分析结果显示,侵犯浆膜[HR=1.490(95%CI:1.154,1.924)]、病理分期Ⅲ期[HR=1.979(95%CI:1.132,3.460)]、淋巴结转移[HR=2.401(95%CI:1.015,5.677)]、miR-223≥4.76[HR=2.140(95%CI:1.063,4.309)]为结肠癌患者预后的危险因素(P<0.05),FBXW7≥1.23[HR=0.625(95%CI:0.475,0.823)]为保护因素(P<0.05)。结论结肠癌组织mi R-223高表达、FBXW7低表达与结肠癌患者病理分期、淋巴结转移及预后有关。

MicroRNA-223及MMP-9在风湿性心瓣膜病合并心房颤动患者中的表达及临床意义

目的探索miRNA-223与金属基质蛋白酶(matrix metalloproteinases,MMP)在风湿性心瓣膜病(风心病)合并心房颤动(房颤)患者的表达水平及在房颤心肌结构重构的发生机制。方法风心病接受瓣膜置换术患者31例,其中风心病窦性心律组15例,风心病慢性房颤组16例。收集患者右心房心肌组织,实时荧光定量聚合酶链反应检测心房肌组织和血清miRNA-223的相对表达量。酶联免疫吸附试验及免疫组织化学检测血清及心肌组织MMP-9蛋白的表达及分布水平;苏木素-伊红染色及Masson染色观察心肌组织病理结构及胶原纤维含量变化。结果与窦性心律组相比,房颤组心房肌组织miRNA-223表达水平升高,差异有统计学意义(0.0603±0.0228 vs.0.0261±0.0035,P<0.01);房颤组血清MMP-9表达水平高于窦性心律组,差异有统计学意义[(4.2281±0.9165)ng/mL vs.(2.7613±1.2166)ng/mL,P<0.05]。MMP-9蛋白表达水平与胶原容积分数(collagen volume fraction,CVF)呈正相关(r=0.406,P<0.05);MiRNA-223表达水平与MMP-9蛋白表达呈正相关(r=0.901,P<0.05)。结论房颤患者心房组织中miRNA-223及MMP-9蛋白表达水平均升高。

miRNA-223、miRNA-21及miRNA-27a与冠心病冠脉病变的关系

目的 探讨miRNA-223、miRNA-21及miRNA-27a与冠心病冠脉病变的关系。方法 选取2021年1月至2022年12月商丘市第一人民医院收治的CHD患者86例为观察组,选取70名同期院内健康体检者作为对照组。对比两组血清miRNA-223、miRNA-21、miRNA-27a水平;分析影响CHD冠脉病变的单因素,采用Logistic回归分析影响CHD冠脉病变的单因素、多因素;对比不同CHD冠脉病变类型的血清miRNA-223、miRNA-21、miRNA-27a水平;对比不同CHD冠脉病变支数的血清miRNA-223、miRNA-21、miRNA-27a水平。结果 观察组miRNA-223、miRNA-21、miRNA-27a表达水平比对照组高,差异有统计学意义(P<0.05);Logistic多因素分析显示,患有高血压、糖尿病以及miRNA-223>1.5、miRNA-21>6.0、miRNA-27a>5.5均是影响CHD冠脉病变的独立危险因素(P<0.05);miRNA-223、miRNA-21、miRNA-27a表达水平:急性心肌梗死>不稳定型心绞痛>稳定型心绞痛,差异有统计学意义(P<0.05);miRNA-223、miRNA-21、miRNA-27a表达水平:三支>双支>单支,差异有统计学意义(P<0.05)。结论 不同冠脉病变CHD患者miRNA-223、miRNA-21、miRNA-27a表达水平不同,提示以上指标对判断CHD患者冠脉病变类型具有一定的临床价值。

转染miR-223模拟物的巨噬细胞结核分枝杆菌清除能力、凋亡、炎症反应变化及miR-223与NLRP3靶向关系

目的 观察肺结核患者血清微小RNA-223(miR-223)水平变化,以及转染miR-223模拟物的巨噬细胞结核分枝杆菌(MTB)H37Rv清除能力、凋亡、炎症反应变化,并分析miR-223与NLRP3靶向关系。方法 选取37例份活动性肺结核患者血清标本(肺结核组)和同期40例健康体检者血清标本(健康组),采用RT-PCR法检测两组血清标本中miR-223。体外培养人单核细胞株THP-1,经佛波脂刺激24 h后分化为巨噬细胞,将巨噬细胞随机分为健康组、MTB组、MTB+mimics-NC组、MTB+miR-223 mimics组,健康组细胞常规培养,MTB组、MTB+mimics-NC组、MTB+miR-223 mimics组均用MTB标准株H37Rv感染巨噬细胞,感染后MTB+mimics-NC组和MTB+miR-223 mimics组应用脂质体转染法分别将mimics-NC、miR-223 mimics转染至细胞中,采用RT-PCR法检测各组细胞miR-223及NLRP3、TNF-α、IFN-γ mRNA,流式细胞术测算各组细胞凋亡率,菌落形成单位(CFU)计数法检测各组H37Rv细菌负荷量。取对数生长期THP-1细胞,随机分为miR-223 mimics+NLRP3-WT组、mimics-NC+NLRP3-WT组、miR-223mimics+NLRP3-MUT组、mimics-NC+NLRP3-MUT组,用Lipofectamine 2000按照试剂盒说明书操作分别将miR-223mimics和NLRP3-WT、mimics-NC和NLRP3-WT、miR-223 mimics和NLRP3-MUT、mimics-NC和NLRP3-MUT共转染至各组细胞,转染后24 h检测各组细胞的相对荧光素酶活性,双荧光素酶报告基因实验验证miR-223与NLRP3是否存在靶向关系。结果 与健康组比较,肺结核组血清miR-223表达降低(P<0.05)。与健康组比较,MTB组miR-223表达、细胞凋亡率降低,NLRP3、TNF-α、IFN-γ mRNA表达及H37Rv细菌负荷量升高(P均<0.05);与MTB+mimics-NC组比较,MTB+miR-223 mimics组miR-223表达、细胞凋亡率升高,NLRP3、TNF-α、IFN-γ mRNA表达及H37Rv细菌负荷量降低(P均<0.05)。双荧光素酶报告基因实验显示,NLRP3是miR-223的靶向基因。结论 肺结核患者血清miR-223表达降低,转染miR-223模拟物能够促进巨噬细胞凋亡,增强MTB感染的巨噬细胞的除菌能力,减轻炎症反应,其机制可能与靶向调控NLRP3有关。

MicroRNA-223在淋巴细胞白血病原代细胞中表达及作用机制的研究

本研究旨在探讨急性淋巴细胞白血病(ALL)、慢性淋巴细胞白血病(CLL)原代细胞中MicroRNA-223与LMO2基因的表达水平及MicroRNA-223的作用机制。应用人淋巴细胞分离液分选ALL、CLL患者及正常人骨髓中淋巴细胞,在ALL、CLL患者骨髓淋巴细胞中转染MicroRNA-223的类似物靶向升高细胞中MicroRNA-223的表达,在正常人骨髓淋巴细胞中转染MicroRNA-223抑制物靶向敲低细胞中MicroRNA-223的表达。转染后培养72 h,用RT-PCR方法检测转染前后MicroRNA-223和LMO2表达量及其相关性,并用流式细胞术进一步观察细胞凋亡和细胞周期的变化。结果表明,转染MicroRNA-223类似物前,ALL、CLL患者中MicroRNA-223表达水平为(433.11±144.88),LMO2水平为(807.10±238.41),正常人转染MicroRNA-223抑制物前,MicroRNA-223表达水平为(949.59±267.39),LMO2的表达为(455.32±176.83);MicrRNA-223的表达在正常人中明显高于ALL、CLL患者(P<0.05),而LMO2的表达在正常人中明显低于ALL、CLL患者(P<0.05)。转染后,ALL、CLL患者中MicroRNA-223表达明显增加(571.86±142.00)(P<0.05),而LMO2表达明显减少(651.97±230.12)(P<0.05);在正常人中MicroRNA-223表达明显降低(646.32±172.93)(P<0.05),LMO2的表达明显升高(541.27±158.86)(P<0.05)。转染后细胞周期及细胞凋亡率的变化表现为,在ALL、CLL患者转染前细胞周期G1/G2细胞比例为(94.75±3.15)%,S期为(5.14±3.12)%;转染后G1/G2细胞比例明显增加(97.03±2.08)%(P<0.05),在S期明显减少(2.97±2.08)%(P<0.05);转染前细胞凋亡率为(54.47±8.72)%,转染后为(60.48±8.81)%,后者明显增加(P<0.05)。正常人转染前细胞周期G1/G2细胞比例是(96.73±2.26)%,S期是(3.25±2.26)%;转染后G1/G2细胞比例明显减少(94.55±2.77)%(P<0.05),在S期明显增加(5.45±2.77)%(P<0.05),细胞凋亡率为(59.02±10.20)%,转染后明显减少(51.96±10.20)%(P<0.05)。结论:淋巴细胞白血病原代细胞中MicroRNA-223表达降低,LMO2表达增高,导致淋巴细胞增殖周期及凋亡异常,这可能是淋巴细胞白血病的发病机制之一。