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.

Distinct Transforming Activity of ABL Family Tyrosine Kinase Oncogenes Is Induced by Their C-Terminal Domain

The TEL/ARG oncogene is similar in structure to the TEL/ABL fusion found in human leukemia, however, we have demonstrated previously that the expression of TEL/ARG in Ba/F3 cells does not sustain strong activity of proliferation, whereas, that of TEL/ABL appeared to induce immediate cell proliferation. To study the molecular basis of the difference in the transforming activity of TEL/ARG and TEL/ABL, TEL/ARG mutants that swapped the kinase domain or C-terminus of ARG with the corresponding domain in ABL were generated, and each mutant was expressed in Ba/F3 cells. A TEL/ARG mutant containing the ABL kinase domain was similar to TEL/ARG in this study, but replacing the ARG C-terminal domain with that of ABL resulted in accelerated proliferation that was similar to that of TEL/ABL. When expressed in primary mouse bone marrow cells by retroviral transduction, spontaneous colony formation in methylcellulose culture was observed, in a fashion dependent on the C-terminal portion of ABL. These results indicate that distinct bio-phenotypes associated with these oncogenes are likely to be regulated by their C-termini, and the C-terminus of ARG contains a functional subdomain that impairs the growth signal induced by ABL family tyrosine kinase.

Malignant pheochromocytoma in neurofibromatosis; mutation screening of RET proto-oncogene, VHL and SDH gene

AIM: To investigate pathogenic mutations related to malignant pheochromocytoma in neurofibromatosis(NF).METHODS: We present a patient with NF and metastatic pheochromocytoma in whom genetic screening for presence of pathogenic mutations in RET protooncogene, von Hippel-Lindau(VHL) and succinate dehydrogenase complex subunits B(SDHB) genes were investigated. RET proto-oncogene mutation screening for exons 10, 11, 13, 14, 15, 16 were examined by polymerase chain reaction(PCR) and direct DNA sequencing in patient. Mutation screening for exons 1, 2, 3 of VHL gene was carried out. Both forward and reverse strandswere subjected to direct sequencing after PCR amplification. The entire coding sequence of SDHB gene was screened for the presence of pathogenic mutations by PCR-sequencing.RESULTS: A 45-year-old man presented with abdominal pain and hypertension over the previous year. The patient was a known case of neurofibromatosis type 1(NF1) who presented at the age of 15 years with hyperpigmented and hypopigmented lesions. After complete evaluation for hypertension, biochemical tests and imagings indicated a malignant pheochromocytoma of 120 mm × 70 mm in size. The patient underwent left adrenalectomy, nephrectomy and splenectomy. After surgery the symptoms improved and blood pressure was controlled. After 5 years he was admitted again for evaluation of hypertensive crisis. Biochemical tests were again consistent with pheochromocytoma and disease relapse. Imaging studies and liver biopsy confirmed metastatic pheochromocytoma to the liver and para-aortic area. 131 Iodine-metaiodobenzylguanidine therapy was carried out. Genetic screening of VHL(exons 1, 2, 3), RET proto-oncogene(exons 10, 11, 13, 14, 15, 16) and SDH complex subunits revealed no pathogenic mutation. CONCLUSION: We conclude that mutations in the NF1 gene are responsible for the patient's clinical findings. However, would be helpful to further examine somatic mutations for a more precise study of genotypephenotype correlation.

C-erbB2、C-erbB3、C-erbB4的表达与卵巢恶性肿瘤的关系

背景与目的:C-erbB2、C-erbB3和C-erbB4均为表皮生长因子受体家族成员,已有的研究表明C-erbB2与卵巢恶性肿瘤的发生、发展相关,但C-erbB3和C-erbB4与卵巢恶性肿瘤的临床病理关系尚未确定,本研究旨在进一步探讨C-erbB2、C-erbB3、C-erbB4表达与卵巢恶性肿瘤的临床病理关系。方法:采用免疫组织化学法对49例卵巢恶性肿瘤,21例卵巢良性肿瘤和19例正常卵巢组织进行C-erbB2、C-erbB3、C-erbB4表达的测定并分析其与临床病理及预后的关系。结果:(1)卵巢恶性肿瘤组织中C-erbB2、C-erbB3、C-erbB4表达阳性率分别为75.51%、69.39%和65.31%,明显高于正常卵巢组织(分别为21.05%、15.79%和21.05%)及卵巢良性肿瘤组织(分别为19.05%、23.81%和23.81%)(P<0.05)。(2)C-erbB2、C-erbB3、C-erbB4的阳性表达率与卵巢恶性肿瘤的组织学类型及分化级别无明显相关性(P>0.05)。(3)临床Ⅲ、Ⅳ期和腹水>500ml的患者肿瘤组织中C-erbB2、C-erbB3、C-erbB4阳性表达率分别为90.0%和91.3%、80.0%和82.6%、93.0%和82.6%,明显高于临床Ⅰ、Ⅱ期和腹水<500ml的患者(P<0.05)。(4)C-erbB2、C-erbB4表达阳性患者的累积生存率明显低于阴性患者的累积生存率(P<0.01);Cox模型分析也表明C-erbB2、C-erbB4为影响卵巢恶性肿瘤患者预后的独立因素。结论:

c-erbB癌基因家族基因扩增与乳腺癌临床病理分期的相关性研究

为探讨c -erbB癌基因家族 4基因扩增与乳腺癌病人临床病理分期的关系及该家族 4基因间的相互作用 ,应用差异聚合酶链反应技术检测 70例乳腺癌组织和癌旁正常乳腺组织中c -erbB家族 4基因扩增情况。结果 70例乳腺癌组织中c-erbB - 1基因和c -erbB - 4基因在癌组织中无扩增 (P >0 0 5) ,而c-erbB - 2基因和c -erbB - 3基因存在明显扩增(P <0 0 5) ,扩增阳性率分别为 33 %和 37%。c -erbB - 2基因扩增阳性率与病理分期正相关 (P <0 0 5) ,c -erbB - 3基因扩增阳性率在乳腺癌病理I至III期中有上升的趋势。同时 ,c -erbB - 2基因扩增与c -erbB - 3基因扩增具有一致性 (P <0 0 0 1 ) ,表明c -erbB - 3基因可能也是乳腺癌发展进程中有用的分子预后指标。对乳腺癌病人检测c -erbB - 2基因与c -erbB - 3基因扩增 。

GLI1介导的巨噬细胞极化调控缺氧性肺动脉高压的作用及机制

目的:探讨神经胶质瘤相关癌基因家族锌指1(GLI1)对缺氧诱导大鼠肺泡巨噬细胞(NR8383)发生M1表型转化的作用机制及对肺动脉高压(PH)进展的影响。方法:将15只成年雄性Wistar大鼠随机分为对照组、缺氧PH模型组和缺氧PH加GANT61给药处理组,每组5只。小动物超声、右心导管实验检测大鼠PH相关指标,确定GLI1特异性抑制剂GANT61对PH进程的影响。HE染色检测肺动脉壁厚度。免疫组化检测α-SMA及M1型极化标志物TNF-α和IL-1β蛋白表达。免疫荧光检测M1型极化标志物CD86及TNF-α表达。Western blot检测GLI1及NF-κB蛋白表达。qRT-PCR检测M1型极化标志物iNOS、CD86、TNF-α、IL-1β及IL-12 mRNA表达。CHIP-PCR验证GLI1调控NF-κB启动子活性。ELISA检测IL-12含量。CCK-8检测大鼠肺动脉平滑肌细胞增殖。结果:GLI1抑制剂GANT61可缓解缺氧大鼠PH(P<0.05)。与缺氧组相比,抑制GLI1可降低大鼠肺组织TNF-α和IL-1β表达(P<0.05)。细胞实验中,缺氧通过上调GLI1激活NF-κB通路诱导NR8383 M1型极化,GLI1过表达促进M1型巨噬细胞相关标志物iNOS、CD86、TNF-α、IL-1β及IL-12表达(P<0.05)。NR8383培养上清可刺激肺动脉平滑肌细胞增殖(P<0.05),参与PH。结论:缺氧通过上调GLI1激活NF-κB通路诱导巨噬细胞发生M1型极化参与PH发生。

A potential oncogenic role of the commonly observed E2F5 overexpression in hepatocellular carcinoma

AIM: To explore the expression pattern of E2F5 in primary hepatocellular carcinomas (HCCs) and elucidate the roles of E2F5 in hepatocarcinogenesis. METHODS: E2F5 expression was analyzed in 120 primary HCCs and 29 normal liver tissues by immunohistochemistry analysis. E2F5-small interfering RNA was transfected into HepG2, an E2F5-overexpressed HCC cell line. After E2F5 knockdown, cell growth capacity and migrating potential were examined. RESULTS: E2F5 was significantly overexpressed in primary HCCs compared with normal liver tissues (P = 0.008). The E2F5-silenced cells showed significantly reduced proliferation (P = 0.004). On the colony formation and soft agar assays, the number of colonies was significantly reduced in E2F5-silenced cells (P = 0.004 and P = 0.009, respectively). E2F5 knockdown resulted in the accumulation of G0/G1 phase cells and a reduction of S phase cells. The number of migrating/invading cells was also reduced after E2F5 knockdown (P = 0.021). CONCLUSION: To our knowledge, this is the first evidence that E2F5 is commonly overexpressed in primary HCC and that E2F5 knockdown significantly repressed the growth of HCC cells.

Expression of c-erbB2 in Gestational Trophoblastic Disease and Its Clinical Significance

Summary: In order to explore a potential indicator of predicting the occurrence and development of gestational trophoblastic tumor, the expression of c-erbB2 oncogene in human normal placenta, hydatidiform mole and choriocarcinoma was investigated. The expression of c-erbB2 was detected immunohistochemically by monoclonal antibody against the gene on the formalin-fixed paraffin sections of 21 hydatidiform moles, 21 invasive moles, 20 choriocarcinomas and 30 normal placentas. Results showed that the expression level of c-erbB2 was significantly higher in gestational trophoblastic tumor than in hydatidiform mole and normal placenta of midterm and term pregnancy (P<0.05), while there was no significant difference between patients with gestational trophoblastic tumor of stage Ⅲ, Ⅳ and those of stage Ⅰ, Ⅱ. It was demonstrated that overexpression of c-erbB2 may closely associated with malignant transformation of hydatidiform mole, not only providing important insight into pathogenesis of gestational trophoblastic tumor, but also having an important significance for the early diagnosis and early treatment of gestational trophoblastic tumor.

Transient receptor potential-related risk model predicts prognosis of hepatocellular carcinoma patients

BACKGROUND Members of the transient receptor potential(TRP)protein family shape oncogenic development,but the specific relevance of TRP-related genes in hepatocellular carcinoma(HCC)has yet to be defined.AIM To investigate the role of TRP genes in HCC,their association with HCC development and treatment was examined.METHODS HCC patient gene expression and clinical data were downloaded from The Cancer Genome Atlas database,and univariate and least absolute shrinkage and selection operator Cox regression models were employed to explore the TRP-related risk spectrum.Based on these analyses,clinically relevant TRP family genes were selected,and the association between the key TRP canonical type 1(TRPC1)gene and HCC patient prognosis was evaluated.RESULTS In total,28 TRP family genes were screened for clinical relevance,with multivariate analyses ultimately revealing three of these genes(TRPC1,TRP cation channel subfamily M member 2,and TRP cation channel subfamily M member 6)to be significantly associated with HCC patient prognosis(P<0.05).These genes were utilized to establish a TRP-related risk model.Patients were separated into low-and high-risk groups based on the expression of these genes,and high-risk patients exhibited a significantly poorer prognosis(P=0.001).Functional analyses highlighted pronounced differences in the immune status of patients in these two groups and associated enriched immune pathways.TRPC1 was identified as a candidate gene in this family worthy of further study,with HCC patients expressing higher TRPC1 levels exhibiting poorer survival outcomes.Consistently,quantitative,immunohistochemistry,and western blot analyses revealed increased TRPC1 expression in HCC.CONCLUSION These three TRP genes help determine HCC patient prognosis,providing insight into tumor immune status and immunological composition.These findings will help design combination therapies including immunotherapeutic and anti-TRP agents.

细胞凋亡的常用调控基因研究近况

细胞凋亡主要受基因的控制 ,现已发现许多基因对细胞凋亡均有直接或间接的调控作用。通常将这些基因分为两大类 ,即细胞生存基因和细胞死亡基因。一般认为与细胞生存有关的基因包括 C- myc、C- abl、Ras、V-src、Bcl- 2 ,EIB,L MW5 - HL,C- kit和 Bcl- x等 ;与细胞死亡有关的基因包含 P35、P53、RB、DCC、WT- 1、Cp Gv、Bcr- abl、V- erb- A、tats2 0、DAD1、 ADO/Fas、 TGF-β、 TRP- 2、 RP- 8、TRPM- 2、SGP- 2、TIA、Bax、ICE、C- rel、irrec-rst等。本文对目前使用较多研究较深入的几种凋亡调控基因 ,即 C- myc基因、Bcl- 2基因、P53基因、ICE基因、Fas基因及 Fas L 和 Cdc2基因的来源、作用和相互间关系的研究近况 ,予以综述 。

家族性非髓样甲状腺癌候选致病基因的研究及展望

家族性非髓样甲状腺癌为一级亲属中有2例或2例以上甲状腺滤泡上皮细胞起源的甲状腺癌患者的家族,并排除甲状腺癌致病因素暴露史。家族性非髓样甲状腺癌是一种常见的肿瘤性遗传病。与散发性非髓样甲状腺癌相比,家族性非髓样甲状腺癌发病年龄更低,发病率更高且转移率更高。因此,一般认为家族性非髓样甲状腺癌的预后更差。尽管已有部分报道,但家族性非髓样甲状腺癌的致病基因尚未明确。全基因组外显子测序技术以其快速、高通量以及低成本而被广泛应用,因此适用于寻找家族性非髓样甲状腺癌的致病基因或易感基因。

多中心腕跗骨骨质溶解综合征一例

多中心腕跗骨骨质溶解综合征(multicentric carpotarsal osteolysis syndrome,MCTO)是一种罕见的常染色体显性遗传病。本文报道1例1岁11月龄患儿肘膝关节屈曲进行性加重,并伴有智力、运动落后,双手及双下肢正位片示多发骨质异常,经基因检测发现肌腱膜纤维肉瘤癌基因同源物B (V-maf musculoaponeurotic fibrosarcoma oncogene family protein B,MAFB)基因c.212C>T (p.P71L)杂合变异,该基因为国外已报道的致病突变,其父母无该基因突变。根据患儿临床表现及基因检测结果诊断为MCTO。同时,对本病进行文献复习,为今后诊断及治疗该类疾病提供借鉴。

癌症与结构基因组学研究

综述了结构基因组学的研究进展,在基因组学水平上对癌症的研究现状及其在癌症研 究中的应用.

家蚕c-Myc基因的全长cDNA克隆及促细胞增殖功能初探

c-Myc是Myc原癌基因家族的重要成员,广泛参与细胞增殖、分化、凋亡等正常生命活动的调节,其异常活化可引发多种肿瘤的发生与发展。基于生物信息学分析和RACE技术,自家蚕5龄幼虫卵巢中克隆了与果蝇d Myc同源的原癌基因Bmc Myc。Bmc Myc基因的c DNA全长1 984 bp,由1 026 bp的完整ORF序列、421 bp的5'-UTR和537 bp的3'-UTR组成,编码蛋白质含341个氨基酸残基,其C末端含有一个Myc家族共有的b HLH保守结构域。Bmc Myc在家蚕各发育时期及5龄第3天幼虫的主要组织中均有表达,不同发育时期以幼虫期和蛹早期的表达水平相对较高。Bmc Myc基因的产物定位于细胞核内,是一种核蛋白因子。在Bm E细胞中表达Bmc Myc出现明显的细胞增殖现象,其下游靶标基因CDK4和ODC的表达亦因之上调,初步证实Bmc Myc基因具有促进细胞增殖的生物学功能。上述结果为进一步阐释Bmc Myc的功能并探索利用其创制蚕丝增产遗传素材提供了理论参考。

MafA真核表达载体的构建及在人肝癌细胞中的表达

目的:构建肌腱膜纤维肉瘤肿瘤基因同系物A(MafA)真核表达载体pEGFP-N2/MafA,pEGFP-C1/MafA,观察MafA在人肝癌细胞HepG-2细胞内的表达。为研究Mafa基因功能和作用机制奠定基础。方法:提取胰腺总RNA,经RT-PCR获得MafA基因片段,在两端分别引入Hind Ⅲ和Sal Ⅰ的酶切位点,重组至有增强绿色荧光蛋白标记的真核表达载体pEGFP-N2,pEGFP-C1中,用脂质体方法转染至人肝癌细胞HepG-2细胞中,通过荧光显微镜观察荧光蛋白的表达,通过RT-PCR检测MafA基因和insulin Ⅱ基因的表达。结果:通过RT-PCR获取了MafA基因并成功克隆入载体,转染的细胞有绿色荧光蛋白表达及MafA基因表达,但没检测到insulin Ⅱ基因表达。结论:成功构建质粒pEGFP-N2/MafA和pEGFP-C1/MafA,并成功表达MafA基因,但没有insulin Ⅱ基因的表达。

小鼠MafB基因重组腺病毒载体的构建及其对破骨细胞分化的影响

目的:构建小鼠肌腱膜纤维肉瘤癌基因B型(MafB)基因重组腺病毒表达载体,阐明MafB对小鼠破骨细胞分化的影响。方法:提取小鼠RAW264.7细胞总RNA,逆转录为cDNA,以cDNA为模板PCR获得目的基因MafB,连接入穿梭质粒pAdTrack-CMV,经酶切鉴定正确的穿梭质粒用PmeⅠ线性化后转化到含pAdEasy-1的大肠杆菌BJ5183菌株中,经PacⅠ线性化后,在HEK 293细胞中包装腺病毒Ad-MafB,感染小鼠RAW264.7细胞,实验分为空白对照组、空载体组(Ad-GFP组)和过表达组(Ad-MafB组),经RT-PCR和Western blotting法检测MafB的表达水平,经抗酒石酸酸性磷酸酶(TRAP)染色、RT-PCR和Western blotting法观察MafB对小鼠可溶性核因子κB受体活化因子配体诱导的破骨细胞分化的影响。结果:与空白对照组和Ad-GFP组比较,Ad-MafB组RAW264.7细胞MafB mRNA表达水平明显升高且蛋白相对表达水平明显增加(P<0.05);TRAP染色,Ad-MafB组TRAP阳性细胞明显少于空白对照组和Ad-GFP组;与空白对照组和Ad-GFP组比较,Ad-MafB组TRAP和组织蛋白酶K(CTSK)mRNA表达降低且蛋白相对表达水平显著降低(P<0.05)。结论:成功构建可在小鼠RAW264.7细胞中过表达MafB的重组腺病毒Ad-MafB,证实MafB可抑制破骨细胞的分化。

神经元素3基因沉默对脐源性胰岛前体细胞MafA表达的影响

目的探讨神经元素3(Ngn3)基因在人脐带间充质干细胞(h UMSCs)向胰岛前体细胞分化过程中的作用以及对肌腱膜纤维肿瘤基因同系物A(MafA)表达的影响。方法组织块法分离培养并鉴定h UMSCs;采用分阶段联合诱导法诱导h UMSCs向胰岛前体细胞分化,将其分为正常诱导组、基因沉默组、空病毒转染组,后两组在诱导第7天分别转染干扰病毒和空病毒,嘌呤霉素筛选后检测感染效果;21 d诱导结束后倒置相差显微镜和电子显微镜观察细胞形态变化;免疫细胞化学技术检测诱导后各组细胞胰岛素、胰高血糖素、Ngn3的表达;Real-time PCR、Western blotting检测Ngn3以及MafA的表达变化。结果成功分离培养h UMSCs;分阶段联合诱导使正常诱导组和空病毒转染组细胞分化为胰岛前体细胞,Ngn3、胰岛素、胰高血糖素呈阳性表达,电子显微镜观察可见分泌颗粒;成功沉默了基因沉默组细胞的Ngn3基因,且该组细胞Ngn3、胰岛素、胰高血糖素呈阴性表达;Ngn3、MafA在基因沉默组明显下降(P<0.05)。结论Ngn3基因沉默阻滞了h UMSCs向胰岛前体细胞的分化,并抑制了MafA的表达。

C/EBPβ通过pim-1介导足细胞损伤的作用机制

目的探讨CCAAT增强子结合蛋白β(C/EBPβ)/丝氨酸/苏氨酸激酶1(pim-1)/NOD样受体热蛋白结构域相关蛋白3(NLRP3)轴介导小鼠肾脏足细胞损伤的作用机制。方法体外培养及转染足细胞后分为Control组、siRNA-NC组(用siRNA-NC转染足细胞)、siC/EBPβ组(用siC/EBPβ慢病毒转染足细胞)、Vector-NC组(空载体转染足细胞)和pim-1-OE组(pim-1过表达慢病毒转染足细胞)。脂多糖(LPS)与腺苷三磷酸(ATP)刺激足细胞后分为LPS+ATP组、LPS+ATP+siRNA-NC组、LPS+ATP+siC/EBPβ组、LPS+ATP+siC/EBPβ+Vector-NC组和LPS+ATP+siC/EBPβ+pim-1-OE组。实时荧光定量PCR(qPCR)检测C/EBPβ和pim-1 mRNA水平。Western blot检测C/EBPβ、pim1、NLRP3、p20半胱氨酸蛋白酶(Caspase)-1、Gasdermin D(GSDMD)、p17白细胞介素(IL)-1β蛋白水平。酶联免疫吸附试验(ELISA)检测炎性因子IL-1β和IL-6水平。染色质免疫共沉淀(chip)实验及双荧光素酶报告基因实验检测C/EBPβ与pim-1基因启动子结合。结果与Control组和siRNA-NC组相比,siC/EBPβ组的C/EBPβ及pim-1 mRNA水平明显下降(P<0.01)。与Control组相比,LPS+ATP组NLRP3、p20Caspase-1、p17IL-1β蛋白水平及IL-1β、IL-6水平明显升高(P<0.01)。与LPS+ATP+siRNA-NC组相比,LPS+ATP+siC/EBPβ组NLRP3、p20Caspase-1、p17IL-1β蛋白水平及IL-1β、IL-6水平降低(P<0.01)。chip实验及双荧光素酶报告基因实验显示C/EBPβ可与pim-1基因启动子结合。与Control组和Vector-NC组比较,pim-1-OE组pim-1 mRNA水平明显升高(P<0.05)。与LPS+ATP+siC/EBPβ+Vector-NC组相比,LPS+ATP+siC/EBPβ+pim-1-OE组NLRP3、p20Caspase-1、p17IL-1β、GSDMD蛋白水平及IL-1β、IL-6水平升高(P<0.05)。结论C/EBPβ/pim-1/NLRP3轴可能参与足细胞损伤,并作为LN治疗的潜在靶点。

基于多数据库分析肝细胞癌组织FAM49B基因水平及其临床意义

目的利用多数据库分析肝细胞癌(HCC)组织FAM49B基因水平及其临床意义。方法利用Oncomine和GEPIA数据库分析HCC组织与正常肝组织FAM49B基因水平,从TCGA获取临床病例资料,应用SPSS 21.0软件统计分析不同临床和病理学特征的HCC组织FAM49B基因水平的异同。自Kaplan Meier Plotter数据库分析不同FAM49B基因水平的HCC患者预后的异同,自MethHC数据库分析FAM49B启动子区甲基化水平,利用String数据库分析与FAM49B相互作用的蛋白网络,采用基因集富集分析(GSEA)预测FAM49B在HCC发病过程中可能的信号调控通路。结果对Oncomine和GEPIA数据库分析显示HCC组织FAM49B基因水平显著高于正常肝组织(P均<0.01);不同性别(P=0.001)、有无肝硬化(P=0.003)、不同肿瘤分化程度(P=0.004)的HCC组织FAM49B基因水平显著不同,而不同年龄、肿瘤大小、病理学分期、甲胎蛋白水平和有无脉管侵犯者无显著性差异(P均>0.05);与FAM49B低水平患者比,FAM49B高水平患者总体生存期显著缩短,具有统计学意义(HR=1.8,P=0.0012);与正常肝组织相比,HCC组织FAM49B启动子区甲基化水平显著降低(P<0.005);与FAM49B相互作用的蛋白有SERPINA1、ISLR和FERMT3;在FAM49B mRNA高水平组织富集到细胞凋亡、细胞周期、调节自噬和P53信号通路等相关基因集(P均<0.05)。结论FAM49B在HCC组织呈高水平,其基因水平与HCC恶性程度和患者不良预后相关,可能作为癌基因在HCC发生发展过程中发挥作用,有望成为HCC诊断及预后评估的新靶点。

FLT3与TET2突变的急性髓系白血病伴IgA-κ型单克隆免疫球蛋白血症1例报告

1病例资料患者男,53岁,因“反复胸闷1个月余”于2020年3月5日就诊于我院。患者入院前1个多月无明显诱因出现胸闷伴心悸,多于劳累后出现,每次持续3~5 min,休息后可缓解,无其他不适。入院后体格检查:生命体征平稳,皮肤黏膜、口唇苍白,皮下无出血点;全身浅表淋巴结未及肿大,胸骨无压痛,双肺呼吸音粗,左肺可闻及哮鸣音,右肺未闻及干、湿性啰音,肝脾肋下未触及。