柞蚕核型多角体病毒ie-2和pe-38基因的克隆与序列分析

采用随机克隆方法,通过对插入pGEM-3Z载体的柞蚕核型多角体病毒基因组的部分片段进行测序和序列分析,获得了柞蚕核型多角体病毒基因组的2个极早期基因ie-2和pe-38的序列及pe-38的5′启动子区,其推定的开放阅读框分别编码295和302个氨基酸,并且内部含有一个保守的锌指结构和亮氨酸拉链。核苷酸和氨基酸同源性比较结果显示:柞蚕核型多角体病毒的ie-2和pe-38基因与黄杉毒蛾多角体病毒的同源性较高,与家蚕核型多角体病毒的同源性都很低;在分子进化方面,这2个基因的保守性不强,出现大片段缺失,是研究分子进化及物种关系比较典型的基因。

Activation of p^(38) mitogen activated protein kinase induced by lipopolysaccharide and its role in TNF a gene expression

Objective: To study the molecular mechanisms of TNF--a expression induced by lipopolysaccharide (LPS) for exploring novel methods to prevent or treat clinical patients with endotoxic shock. Methods:Protein kinase assay was used to detect the kinase activity stimulated by LPS; Con focal laser scan technique was used to show the translocation of p38 on the activation; RT PCR and reporter gene system were used to study the molecular mechanism of TNF -a gene transcription. Results: In RAW cells it was found that p38 was activated on the stimulation of LPS. and activated p38 moved into nucleus from cytosol; TNF--a mRNA increased on the stimulation of LPS and the increased promoter transactivity induced by LPS could be inhibited significantly by specific inhibitor for p38. Conclusion: p38 mitogen activated protein kinase (MAPK ) was activated by the stimulation of LPS,which brought about its entry to the nucleus to act on transcription factors to regulate cellular processes. p38 MAPK Is an important regulator of TNF--a gene expression induced by LPS.

葡萄扇叶病毒杭州分离物(GFLV-H)P_(38)蛋白基因克隆及序列分析

为了证实GFLV-HP38蛋白的性质及其在寄主扩散中的作用,根据葡萄扇叶病毒(Grapevinefanleafvirus,GFLV)法国分离物F13RNA2序列合成特异性引物,利用RT-PCR从GFLV-H基因组中扩增出P38蛋白基因的cDNA片段,并克隆到pGEM-T-easyvector上。序列分析表明该基因包含1044个核苷酸,编码347个氨基酸。序列比较发现GFLV-HP38蛋白基因与GFLV-F13对应基因核苷酸和氨基酸的同源性分别为90%和96%;与线虫传多面体病毒属中的南芥菜花叶病毒(Arabismosaicvirus,ArMV)和番茄环斑病毒(Tomatoringspotvirus,TomRSV)对应基因氨基酸同源性分别为85%和38.6%,与烟草黑环病毒(Tabaccoblackringvirus,TBLV)、葡萄铬色花叶病毒(Grapevinechromemosaicvirus,GCMV)和树莓环斑病毒(Raspberryringspotvirus,RRSV)的同源性均低于30%。

肺腺癌组织中RNA结合基序蛋白38和p53基因的表达及其临床意义

目的:分析肺腺癌组织中RNA结合基序蛋白38基因(RNA-binding motif protein 38,RBM38)及抑癌基因p53 m RNA和蛋白的表达情况,探讨其在肺腺癌发生发展中的意义。方法:取2012年10月至2015年6月新疆医科大学附属肿瘤医院收治的50例肺腺癌患者的肿瘤组织标本作为实验组,相对应的癌旁组织标本作为对照组。用RT-PCR法检测两组中RBM38及p53m RNA相对表达量,用Western blotting法检测两组中RBM38及p53蛋白的相对表达量。结果:实验组RBM38 m RNA及蛋白相对表达量(0.357±0.170、0.294±0.149)均高于对照组(0.271±0.128、0.206±0.099),实验组p53 m RNA及蛋白(0.457±0.208、0.671±0.200)相对表达量均高于对照组(0.308±0.167、0.332±0.071),差异均有统计学意义(均P<0.01)。RBM38表达与肺腺癌患者TNM分期、浸润深度有关(P<0.05),p53表达与患者TNM分期有关(P<0.05)。实验组RBM38与p53蛋白表达呈负相关(r=-0.626,P<0.01)。结论:肺腺癌组织RBM38、p53 m RNA及蛋白表达均高于癌旁组织,两者均与患者TNM分期等病理参数关系密切。随着RBM38蛋白表达的增加p53蛋白随之减少,RBM38可能通过抑制p53的翻译从而促进肺癌的发生发展,RBM38可能成为肺腺癌分子靶向治疗的靶点。

二化螟两种P450基因CYP4M38和CYP4M39的时空表达分析

细胞色素P450在昆虫对外源物质代谢中发挥重要作用,是昆虫重要的解毒酶系。CYP4家族是昆虫细胞色素P450基因家族中的重要分支,与昆虫的解毒代谢密切相关。为初步明确CYP4家族基因在二化螟中的表达信息,本文测定分析了二化螟两种P450基因CsCYP4M38和CsCYP4M39的序列同源性及时空表达谱,序列同源性分析发现CsCYP4M38与烟草天蛾MsCYP4M2氨基酸序列同源性最高,序列一致性高达56.86%;CsCYP4M39与烟草天蛾MsCYP4M1氨基酸序列同源性最高,序列一致性高达59.96%,构建系统发育树显示,CsCYP4M38与CsCYP4M39属于CYP4家族,且分别与MsCYP4M2和MsCYP4M1进化距离较近;时空表达谱测定结果表明,两种基因在不同发育阶段和不同组织中的表达存在差异性,CsCYP4M38在2龄幼虫、5龄幼虫及雌成虫内表达量相对较高,在1龄幼虫中表达量最低,CsCYP4M39在幼虫期表达量相对较高,且表达量随龄期增加呈现先上升后下降的趋势,在卵、蛹及成虫中表达量相对较低。CsCYP4M38和CsCYP4M39在脂肪体、中肠及表皮中的表达量相对较高,且均在脂肪体内的表达量最高。明确基因表达谱是研究其功能的基础,CsCYP4M38和CsCYP4M39在不同阶段的表达量具有一定的变化性,说明这两种基因在二化螟不同发育历期中的功能不同,而两种基因均在脂肪体中表达量最高,这可能与脂肪体是昆虫的主要的解毒代谢场所有关。

棉花GhSEDEG38基因调控棉花耐盐性的功能分析

基于棉花体细胞胚胎再生不同时期表达谱中筛选出一系列差异表达转录因子,通过RT-PCR和qRT-PCR分析这些转录因子在不同逆境处理下的表达,发现GhSEDEG38基因(somatic embryogenesis differencially expressed gene 38)的表达受盐胁迫诱导明显上调;序列分析发现GhSEDEG38编码bZIP型转录因子,与拟南芥bZIP53基因同源。为进一步验证该基因的功能,构建了该基因的RNAi干涉载体并转化棉花,通过分子检测获得了表达量显著降低的转基因棉花株系。通过对萌发期和三叶期转基因材料和对照材料进行盐处理发现,干涉GhSEDEG38基因降低棉花在萌发期及苗期对盐胁迫的抗性,盐处理后转基因植株的MDA含量和活性氧含量显著高于对照材料,而可溶性糖含量显著低于对照材料。综上,GhSEDEG38参与棉花对盐胁迫的应答。

Senescence in adipose-derived stem cells and its implications in nerve regeneration

Adult mesenchymal stem cells, specifically adipose-derived stem cells have self-renewal and multiple differentiation potentials and have shown to be the ideal candidate for therapeutic applications in regenerative medicine, particularly in peripheral nerve regeneration. Adipose-de- rived stem cells are easily harvested, although they may show the effects of aging, hence their potential in nerve repair may be limited by cellular senescence or donor age. Cellular senescence is a complex process whereby stem cells grow old as consequence of intrinsic events （e.g., DNA damage） or environmental cues （e.g., stressful stimuli or diseases）, which determine a permanent growth arrest. Several mechanisms are implicated in stem cell senescence, although no one is exclusive of the others. In this review we report some of the most important factors modulating the senescence process, which can influence adipose-derived stem cell morphology and function, and compromise their clinical application for peripheral nerve regenerative cell therapy.

高产油绿球藻GIEC-38转录本和基因表达谱分析

通过对天然条件下生长好且含油高的绿球藻(Chlorococcum sp.) GIEC-38细胞内转录本的测定,发现:在获得的74 605条转录本、65 984个基因中共得到344条代谢途径,其中核糖体、蛋白质、核苷酸、核糖核酸、碳固定、光合作用以及脂代谢等通路都非常活跃。通过缺N培养发现GIEC-38含油脂可达50%以上,通过对比细胞表达谱发现相比于原始藻株,缺N条件下培养的GIEC-38细胞中有868个基因显著上调、1 157个基因显著下调,分布在41个生物学功能、71条代谢途径中。其中,为脂肪酸的合成提供大量原料的中间产物合成酶,以及脂类代谢相关的几个通路中关键酶的基因,表达都有明显上调,促使细胞脂类的合成,提高了细胞的油脂产量。

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.

深圳地区类风湿关节炎患者IL-17A基因rs2275913位点多态性与血清中IL-17A,IL-38水平表达的相关性研究

目的了解深圳地区类风湿关节炎(Hieumatord arthritis,RA)患者IL-17A基因rs2275913位点多态性与血清中IL-17A,IL-38水平表达的相关性。方法选择103例RA患者作为RA组,另选取116例非RA健康人群作为对照组。分别检测IL-17A,IL-38及类风湿因子(rheumatoid factors,RF)水平,同时对IL-17A基因rs2275913位点多态性进行分析。结果RA组IL-17A和RF水平(54.06±1.87 pg/ml和29.65±4.02 IU/ml)明显高于对照组(33.29±1.42 pg/ml和5.27±1.38 IU/ml),而IL-38水平(40.92±8.67 pg/ml)明显低于对照组(53.78±12.04 pg/ml),两组差异有统计学意义(t=7.2065,18.2972,5.0197,均P<0.05)。RA组随着病情活动度的加重IL-17A和RF水平明显升高,而IL-38水平明显降低,不同活动度之间差异均有统计学意义(F=12.5271,7.9351,9.2702,均P<0.05)。RA组IL-17A基因rs2275913位点AA基因型和A等位基因检出率(47.57%和63.11%)明显高于对照组(15.52%和30.60%),两组差异有统计学意义(χ^(2)=5.9256,4.0272,均P<0.05)。RA组AA基因型IL-17A水平比AG和GG基因型明显升高,而IL-38水平明显降低,不同基因型之间差异有统计学意义(F=7.0625,5.1873,P均<0.05),但不同基因型RF水平差异无统计学意义(F=1.0961,P=0.1205)。经Spearman相关性分析,RA组IL-17A水平与RF水平呈正相关,而与IL-38水平呈负相关(r=0.5012,-0.6924,均P<0.05)。结论RA组IL-17A水平明显升高,且随病情活动度加重而升高。同时IL-17A基因rs2275913位点多态性与深圳地区RA发病的易感性相关,其中AA基因型可能是RA发病的易感危险基因之一。

CD38表达对成人BCR/ABL融合基因阳性急性B淋巴细胞白血病预后的影响

目的:探讨急性B淋巴细胞白血病(B-ALL)患者白细胞分化抗原38(CD38)表达与疗效及预后的关系。方法:收集2014年至2017年在我院初诊的B-ALL患者共74例,用流式细胞仪检测患者骨髓白血病细胞免疫表型,实时荧光定量PCR检测断裂点簇基区-Abelson酪氨酸激酶(BCR-ABL)融合基因。分别依据CD38表达强度分为CD38^+组和CD38-组以及BCR-ABL融合基因存在与否分为BCR-ABL^+组和BCR-ABL-组,回顾性分析不同组别患者的临床资料及预后。结果:74例B-ALL患者中,CD38^+组和CD38-组患者分别为34例及40例,BCR-ABL^+组和BCR-ABL-组分别为30例及44例。BCR/ABL^+组患者CD38表达率显著低于BCR/ABL-组(26.7%vs 73.3%,P=0.017)。CD38^+和CD38-患者的总生存期(OS)及无进展生存期(PFS)差异无统计学意义。BCR/ABL^+患者中,CD38^+组的中位OS和PFS显著低于CD38-组(15.73个月vs 25.8个月,9.27个月vs 25.8个月;分别P=0.01和P=0.021);而BCR/ABL-患者中,CD38^+组和CD38-组的中位OS和PFS差异均无统计学意义。结论:CD38表达是BCR/ABL^+ALL患者预后不良的因素,即使酪氨酸酶抑制剂(TKI)治疗也不能改变这种不良预后。

西安市采暖季与非采暖季PM2.5染毒的人胚肺细胞基因差异表达研究

目的寻找与大气污染致病相关的相关基因,为阐明大气污染致病的生物学机制提供科学依据。方法采用mRNA斑点杂交鉴定技术,克隆经采暖季≥75μg/m3 PM2.5与非采暖季<75μg/m3 PM2.5染毒的WI-38人胚肺细胞,分析其间的基因表达差异。放免法测定炎性因子TNF-α、IL-2、IL-6和IL-8。结果与对照组比较,PM2.5>100μg/mL染毒24h后,WI-38人胚肺细胞细胞因子TNF-α、IL-6和IL-8明显升高,IL-2明显减低(P<0.05)。不同浓度PM2.5处理的WI-38人胚肺细胞间差异表达的基因片段,可见48份基因样本在350bp处出现清晰条带;该48份基因样本经斑点杂交后,Tester cDNA杂交的48个斑点中,41份可见黑褐色斑点,而同样样本与Driver cDNA杂交的该48份样本均未见明显显色。结论 PM2.5能诱导WI-38人胚肺细胞产生炎性损伤,≥75μg/m3 PM2.5染毒的WI-38人胚肺细胞存在明显的基因损伤。

The enhancement effect of pp38 gene product on the activity of its upstream bi-directional promoter in Marek's disease virus

There was a bi-directional promoter between gene 38 kd phosphorylated protein (pp38) gene; 1.8-kb mRNA transcript gene family in the genome of Marek's disease virus (MDV). In this study, enhanced green fluorescence protein (EGFP) reporter plamids, pP(pp38)-EGFP; pP(1.8-kb)-EGFP, were constructed under this bi-directional promoter in two directions. The two plasmids were transfected into uninfected chicken embryo fibroblast (CEF), MDV clone rMd5 infected CEF (rMd5-CEF); pp38-deleted derivative rMd5Δpp38 infected CEF (rMd5Δpp38-CEF) respectively. Transfection analysis showed that EGFP was only expressed in rMd5-CEF,; no EGFP could be detected in uninfected CEF or rMd5Δpp38-CEF, implying that pp38 was a factor influencing the activity of the promoter. The pp38-expressing recombinant plasmid pcDNA-pp38 was constructed to co-transfect CEF or rMd5Δpp38-CEF with pP(pp38)-EGFP or pP(1.8-kb)-EGFP. In this case, EGFP could be detected only in rMd5Δpp38-CEF but still not in uninfected CEF, implying that pp38 needs other protein(s) to work together for the complete trans-acting activity. Another MDV gene, 24 kd phosphorylated protein pp24 gene was cloned into pcDNA3.1 as a pp24-expressing recombinant plasmid pcDNA-pp24. When uninfected CEF was co-transfected with pcDNA-pp38, pcDNA-pp24; EGFP expressing plasmids pP(pp38)-EGFP or pP(1.8-kb)-EGFP, the EGFP could be detected. These results indicated that pp38; pp24 could enhance the activity of the promoter when they worked together. DNA mobility shift assay showed that pp38 would bind to the bi-directional promoter with the co-existing of pp24, although neither of them alone influenced mobility of the promoter DNA. All the above suggested that MDV pp38 could transactivate the bi-directional promoter when combined with pp24. The results also indicated that the activity of the promoter in the direction of 1.8-kb mRNA was significantly stronger than that of pp38 direction.

某市2109例女性宫颈细胞中HPV基因型别的研究

目的人乳头瘤病毒(HPV)感染是宫颈上皮内瘤变及宫颈癌的主要致病原因。本文旨在探讨深圳市女性宫颈细胞中23种HPV感染的基因型分布情况。方法从深圳市妇幼保健院体检中心的2109例女性宫颈上皮细胞标本中提取23种HPVDNA,采用基因扩增及基因芯片技术对其宫颈细胞中的23种HPV基因型别进行检测,并对受检者的感染情况进行分析。结果 2109例女性宫颈上皮细胞标本中检出HPV感染者446例,总的HPV感染率为21.15%(446/2109),其中单一型别的阳性检出率为15.32%(323/2109);单一型别的感染中HPV52型为47例,其阳性检出率为2.23%(47/2109),其次是HPV43和58型均为38例,其阳性检出率均为1.80%(38/2109),是单一型别感染中最主要的型别。混合型HPV感染123例,其阳性检出率为5.83%(123/2109);其中HPV16+43、HPV16+58型各5例,均占混合型感染的4.07%(5/123),其次是HPV43+52、HPV43+56、HPV43+66型的二重感染各3例,均占混合型感染的2.44%(3/123),是混合型感染的主要型别。结论 HPV43、HPV52、HPV58单一型别及HPV16+43和HPV16+58型是感染深圳市女性宫颈细胞的主要基因型别,基因芯片检测技术可应用于宫颈细胞标本,一次可检测23种HPV基因型别,特异性强,敏感性高,对中国女性宫颈HPV感染基因型的分子流行病学的调查研究具有重要的意义。

A Neurobiological Examination of Environmental, Subjective, Peripheral and Central Taste Sensation Processing Variances Associated with Taste Alterations: A Case Study Method

This study examines a common phenomenon that is greatly ignored by the clinical community for numerous reasons. Many people for a multitude of reasons experience taste alterations. The supertaster phenomenon is an alteration of taste that requires more investigation. In this study, a proband was examined for subjective reports of a taste alteration to determine its nature through a medical history examination and interview as well as any recollections of the taste disorder in her life. Through this examination, it was found that medical history examination and interview of the proband that many members of her nuclear family showed traits of the same taste disorder or in the case of one family member being a suspect for the taste alteration and one member not showing any signs because of genetic diversity as a half-sibling. Taste disorders are heritable, have multiple health and mental health consequences, influence life choices including mate choice, avoidance behaviors, social choices, alcohol use/abuse, smoking, food choices, and more. More awareness is needed in the research and clinical community into taste alterations as well as calls for future research from neuroscience, biomedical science, life science, and allied science community to investigate taste alterations.

人白细胞介素-38基因的克隆及序列分析

目的:克隆人IL-38基因全长编码区cDNA,并对其进行序列分析。方法:从人皮肤组织中提取总RNA,逆转录为cD-NA,用热启动PCR方法,扩增人IL-38基因的编码区cDNA,通过限制性内切酶酶切后,定向插入pcDNA3.1质粒载体,构建真核表达质粒载体pcDNA3.1-hIL-38,然后进行酶切鉴定与序列分析。结果:人IL-38基因的PCR产物和重组载体经凝胶电泳和酶切鉴定、序列分析证实,其序列与GenBank中数据一致。人IL-38基因的全长编码序列为459 bp,编码152个氨基酸。结论:成功的克隆了人IL-38基因并构建了其真核表达质粒载体,为以后深入研究IL-38的生物学功能奠定了物质基础。

结核分枝杆菌38ku蛋白的制备及其抗原性研究

目的基因克隆、表达、纯化结核分枝杆菌38ku蛋白,研究其抗原性,评价其在血清学诊断中的价值。方法2003年2月至2004年3月在中国药品生物制品检定所菌苗室以结核分枝杆菌H37Rv基因组DNA为模板,通过聚合酶链反应(PCR)方法对38ku蛋白基因进行扩增,以PET-30a(+)为载体构建重组质粒,在大肠埃希菌中表达38ku蛋白,通过金属离子螯合亲和层析方法纯化重组蛋白,免疫印迹和酶联免疫吸附试验(ELISA)方法分析该重组蛋白的抗原性。结果构建了具有正确基因序列的38ku蛋白重组质粒,在大肠埃希菌BL21(DE3)中以包涵体形式表达,经过一步金属离子螯合亲和层析后得到纯度为92.7%的目的蛋白。免疫印迹试验结果表明该蛋白能与羊抗结核血清发生特异免疫结合反应。应用ELISA方法对结核血清参考品进行检测,敏感度和特异度分别为80.5%(33/41)和96.0%(25/26)。结论大肠埃希菌工程菌以包涵体的形式表达38ku蛋白,该蛋白具有良好的免疫原性,可望成为结核血清学的诊断抗原之一。

Analyzing the H19-and T65-epitopes in 38 kd phosphory-lated protein of Marek's disease viruses and comparing chicken immunological reactions to viruses point-mutated in the epitopes

DNA sequencing analysis in 38 kd phosphorylated protein (pp38) ORF of Marek's disease viruses (MDV) indicated that all tested 10 virulent strains with different pathotypes had 'A' at base #320 and glutamine at aa#107 while reacted with monoclonal antibody (Mab) H19 in indirect fluorescence antibody test (IFA). However, vaccine strain CVI988 had 'G' at base#320 and arginine at aa#107 instead, when it was negative in IFA with Mab H19. Some strains were also reactive with Mab T65 in IFA while there was 'G' at base #326 and glycine at aa#109, but the other strains, which had 'A' at base #326 and glutamic acid at aa#109, did not react with Mab T65. By comparison of CVI988 to its point mutants CVI/rpp38(AG) and CVI/rpp38(AA) with 1 or 2 base(s) changes at bases #320 and /or #326 of pp38 gene for their reactivity with Mab H19 and T65, it was confirmed that the glutamine at aa#107 and glycine at aa#109 were critical to epitopes H19 and T65 respectively. Immuno-reactions to MDV were compared in SPF chickens inoculated with cloned CVI988 and its mutant CVI/rpp38(AG). It was found that antibody responses to MDV in chickens inoculated with CVI/rpp38(AG) were delayed and significantly lower than that in chickens inoculated with the native CVI988. By differential comparison of antibody titers to different antigens, a third epitope specific to CVI988 and dependent on arginine at aa#107 was suggested to be responsible for the big difference in antibody responses induced by native CVI988 and its mutant.

Effect of PRAK gene knockout on the proliferation of mouseembryonic fibroblasts

p38 regulated/activated protein kinase(PRAK)plays a key role in cell senescence and tumor suppression.The aim of this study was to investigate if PRAK had effect on cell proliferation.The growth of PRAK+/+and PRAK^(–/–)mouse embryonicfibroblast(MEF)cells was measured by methylthiazoletetrazolium(MTT)colorimetric assay,and the proportion of the cell number in different phases of the cell cycle was analyzed byflow cytometry.The growth curves showed that the growth rate was notably decreased,and cell double time was elongated in PRAK^(–/–)cells;moreover,the number of PRAK^(–/–)cells was decreased by 44.5%compared with that of PRAK+/+cells cultured for 96 h,suggesting that G2/M transition is inhibited in PRAK^(–/–)cells.Meanwhile,G1/S transition was also inhibited in PRAK^(–/–)cells,observed withflow cytometry analysis.The ratios of G0/G1,G2/M,and S phases of PRAK+/+cells were 44.9%,12.2%,and 42.9%,respec-tively,while those of PRAK^(–/–)cells were 55.3%,7.3%,and 37.4%,respectively.There were 23.1%increase and 12.7%decrease of the number of PRAK^(–/–)cells in G1 and S phases in comparison with that of PRAK+/+cells,respectively.Taken together,PRAK gene knockout in MEF cells leads to cell cycle arrest and proliferation inhibition.

全面发育迟缓1例患儿 EEF1A2基因的变异分析

目的总结EEF1A2变异所致常染色体显性复杂神经发育障碍患儿的临床表现并分析其致病机制。方法以2021年7月就诊于洛阳市妇幼保健院的1例全面发育迟缓患儿作为研究对象。回顾分析患儿的临床资料,对其进行全外显子组检测,并复习相关文献。本研究通过了洛阳市妇幼保健院医学遗传与产前诊断医学伦理委员会的审查(批准号:YCCZ-KS-KY-2021-03)。结果患儿为女性,2岁4个月,表现为全面发育迟缓、步态不稳、四肢肌力偏低、无语言发育。其父母身体健康,否认相关家族遗传病史。基因检测发现患儿携带EEF1A2基因(NM_001958.5)c.44A>G(p.H15R)新发杂合错义变异,既往未见报道,根据美国医学遗传学与基因组学学会相关指南判定为可能致病性。结论EEF1A2基因c.44A>G(p.H15R)变异可能是患儿的遗传学病因。上述发现丰富了EEF1A2基因的变异谱。