Development of a Rapid Multi-residue Assay for Detecting β-lactams Using Penicillin Binding Protein 2x

Objective To develop a rapid multi-residue assay for detecting 16 demanded by the European Union （EU）. Methods A recombinant penicillin-binding protein （PBP） 2x＊ from Streptococcus pneumoniae R6 was expressed in vitro and six β-1actams were conjugated to HRP by four methods. A rapid multi-residue assay for β-1actams was established with PBP2x＊ and HRP-conjugate. Results PBP2x＊ was expressed and purified successfully and the ideal HRP-conjugate was identified. The multi-residue assay was developed. After optimization, penicillin G, ampicillin, amoxicillin, cloxacillin, dicloxacillin, oxacillin, nafcillin, cephalexin, ceftiofur, cefalonium, cefquinome, cefazolin, cefoperazone, cephacetrile, and cephapirin can be detected at levels below MRL in milk with simple pretreatment. Conclusion This assay developed can detect all 16 β-1actams demanded by the European Union （EU）. The whole procedure takes only 45 min and can detect 42 samples and the standards with duplicate analysis.

Reduction of Beta-Lactam Antimicrobial Activity in <i>Staphylococcus aureus</i>Abscesses by Neutrophil Alteration of Penicillin-Binding Protein 2

We previously demonstrated that brief nonkilling neutrophil exposure diminishes the binding affinity of S. aureus penicillin-binding protein (PBP) 2. We sought to investigate further the role of the neutrophil in the alteration of antimicrobial activity and its interaction with PBP-2 by studying the activity of cefotaxime, which highly binds to PBP 2, and cephalexin, which minimally binds to PBP 2. Using S. aureus, cultured in vitro in sterile-filtered normal and neutrophil depleted abscess fluid, we sought to demonstrate an in vivo significance of the neutrophil effect upon the activity of antimicrobials that target PBP-2 by studying the same antimicrobials in an experimental S. aureus abscess. Rats were implanted with perforated tissue cages and infected with S. aureus;some rats were neutrophil depleted by mechlorethamine. Abscess fluids from normal and neutropenic abscesses were harvested, pooled, sterile-filtered and stored for the time-kill studies. Treatment studies were performed by administering either 300 μg/kg/d cefotaxime or cephalexin for 7 days in other rats with 24 hour-old tissue-cage S. aureus abscesses. In time-kill studies, cefotaxime was highly active against stationary phase S. aureus in MHB and in neutropenic abscess fluid, but less active in the non-neutropenic abscess fluid (p 10 kill, p = 0.029 vs. 0.81 ± 2.5, p = NS). These data suggest that neutrophil exposure, which diminishes S. aureus PBP-2 binding affinity [or total quantity], also adversely affects the antimicrobial activity of cefotaxime, which binds to PBP-2, as compared to cephalexin. Altered PBP targets from neutrophil exposure may be a mechanism of antimicrobial resistance within abscesses.

A Cdc2-related protein kinase hPFTAIRE1 from human brain interacting with 14-3-3 proteins

hPFTAIRE1 （PFTK1）, a Cdc2-related protein kinase, is highly expressed in human brain. It exhibits cytoplasmic distribution in Hela cells, although it contains two nuclear localization signals （NLSs） in its N-terminus. To search for its substrates and regulatory components, we screened a two-hybrid library by using the full-length hPFTAIRE1 as a bait. Four 14-3-3 isoforms （β,ε,η,τ） were identified interacting with the hPFTAIRE1. We found a putative 14-3-3 binding consensus motif（RHSSPSS） in the hPFTAIRE 1, which overlapped with its second NLS. Deletion of the RHSSPSS motif or substitution of Ser^119 gwithAla in the conserved binding motif abolished the specific interaction between the hPFTAIRE 1 and the 14-3 -3 proteins. The mutant S 120A hPFTAIRE1 also showed a weak interaction to the 14-3-3 proteins. The results suggested that the Ser^119 is crucial for the interaction between hPFTAIREI and the 14-3-3 proteins. All the hPFTAIRE1 mutants distributed in cytoplasm of Hela cells and human neuroblastoma cells （SH-SY5Y） when fused to the C-terminus of a green fluorescent protein （GFP）, indicating that binding with the 14-3-3 proteins does not contribute to the subcellular localization of the hPFTAIRE1, although the binding may be involved in its signaling regulation.

Exosomes derived from microglia overexpressing miR-124-3p alleviate neuronal endoplasmic reticulum stress damage after repetitive mild traumatic brain injury

We previously reported that miR-124-3p is markedly upregulated in microglia-derived exosomes following repetitive mild traumatic brain injury.However,its impact on neuronal endoplasmic reticulum stress following repetitive mild traumatic brain injury remains unclear.In this study,we first used an HT22 scratch injury model to mimic traumatic brain injury,then co-cultured the HT22 cells with BV2 microglia expressing high levels of miR-124-3p.We found that exosomes containing high levels of miR-124-3p attenuated apoptosis and endoplasmic reticulum stress.Furthermore,luciferase reporter assay analysis confirmed that miR-124-3p bound specifically to the endoplasmic reticulum stress-related protein IRE1α,while an IRE1αfunctional salvage experiment confirmed that miR-124-3p targeted IRE1αand reduced its expression,thereby inhibiting endoplasmic reticulum stress in injured neurons.Finally,we delivered microglia-derived exosomes containing miR-124-3p intranasally to a mouse model of repetitive mild traumatic brain injury and found that endoplasmic reticulum stress and apoptosis levels in hippocampal neurons were significantly reduced.These findings suggest that,after repetitive mild traumatic brain injury,miR-124-3 can be transferred from microglia-derived exosomes to injured neurons,where it exerts a neuroprotective effect by inhibiting endoplasmic reticulum stress.Therefore,microglia-derived exosomes containing miR-124-3p may represent a novel therapeutic strategy for repetitive mild traumatic brain injury.

早期胃癌患者Hp感染情况与转化生长因子-β_(1)、青霉素结合蛋白1A表达的关系

目的探讨早期胃癌患者幽门螺杆菌(Hp)感染情况与转化生长因子-β_(1)(TGF-β_(1))、青霉素结合蛋白1A(PBP1A)表达水平的关系。方法选取2020年1月—2023年1月在铜川市人民医院接受手术治疗,并经过病理检查确诊为早期胃癌的106例患者。将合并Hp感染患者作为阳性组,未感染Hp患者作为阴性组,分别有49和57例。收集患者的一般资料和病理特征,并比较两组术前血清中炎症因子[白细胞介素-6(IL-6)、IL-8、肿瘤坏死因子-α(TNF-α)]及TGF-β_(1)水平。术后检测患者肿瘤组织中PBP1A的表达情况。采用多因素一般Logistic回归模型分析早期胃癌患者Hp感染与TGF-β_(1)、PBP1A水平的关系,并通过受试者工作特征(ROC)曲线评估TGF-β_(1)、PBP1A对早期胃癌患者Hp感染情况的诊断效能。结果两组患者性别构成、年龄、体质量指数、家族疾病史、肿瘤直径和部位、肿瘤类型、分期和淋巴结转移率的比较,差异均无统计学意义(P>0.05)。阳性组肿瘤低分化、浸润程度至黏膜下层的患者数均较阴性组多(P<0.05)。阳性组IL-6、IL-8、TNF-α及TGF-β_(1)水平均较阴性组高(P<0.05),PBP1A mRNA水平较阴性组低(P<0.05)。多因素一般Logistic分析,结果显示:肿瘤低分化[OR=6.345(95%CI:1.571,25.630)]、高浸润性[OR=7.853(95%CI:1.824,33.805)]、高TGF-β_(1)水平[OR=1.541(95%CI:1.287,1.844)]、低PBP1A mRNA水平[OR=0.003(95%CI:0.000,0.179)]是患者感染Hp的危险因素(P<0.05)。ROC曲线结果显示,TGF-β_(1)联合PBP1A在早期胃癌患者Hp感染的诊断中的曲线下面积为0.921,敏感性为81.6%(95%CI:0.680,0.912),特异性为86.0%(95%CI:0.742,0.937)。联合诊断的准确性高于单独指标检测。结论TGF-β_(1)与PBP1A在Hp感染的早期胃癌患者中有较高的评估价值,可作为患者的诊断和预后的参考。

多重耐药鲍曼不动杆菌β-内酰胺酶、膜孔蛋白及β-内酰胺类靶位编码基因研究

目的研究一株多重耐药鲍曼不动杆菌(Multi-drug-resistant Acinetobacter baumannii,MDR-ABA)J65可能存在的β-内酰胺类药物耐药机制。方法 MDR-ABA J65株分离自2011年12月某三甲医院住院患者痰标本,用gyrA和parC基因PCR扩增、测序和BLASTn比对确认菌种。用PCR法分析该菌株的PBP1a、PBP2、CarO和33种A^D类β-内酰胺酶编码基因,并对检出的β-内酰胺酶编码基因作了插入序列与β-内酰胺酶编码基因连锁检测。结果 MDR-ABA J65检出β-内酰胺酶编码基因bla TEM-1、bla ADC-62、bla OXA-23、bla OXA-66,插入序列与β-内酰胺酶编码基因连锁检测显示ISaba1-ADC-62和ISaba1-OXA-23为阳性。PBP1a、PBP2和CarO编码基因序列与鲍曼不动杆菌敏感株(SDF)相比均存在有义突变,且三维结构同源建模显示,与SDF株PBP1a、PBP2和CarO蛋白分子立体结构有明显差别。结论 MDR-ABA J65对β-内酰胺类耐药机制为PBPs和孔蛋白CarO变异及可移动遗传元件介异的β-内酰胺酶编码基因。

β-内酰胺抗生素作用机制的研究进展

以青霉素为代表的β-内酰胺类抗生素,在人类征服细菌感染的70多年历史中起着不可或缺的重要作用;β-内酰胺类抗生素作用机制的研究,为这类抗生素品种的开发以及在临床上的合理应用起到了重要的作用。本文简要阐述了这类抗生素作用机制的有关研究脉络和成果,特别是近年来新技术新方法的应用在该领域所取得的进展,以及在真正解析抗菌机制研究方面对学术界提出的挑战。

鲍曼不动杆菌耐氨苄西林-舒巴坦与青霉素结合蛋白基因变异的相关性

目的测定鲍曼不动杆菌临床分离株对常用抗菌药物的敏感性;分析青霉素结合蛋白(PBP)基因的变异,探索其与鲍曼不动杆菌对氨苄西林-舒巴坦耐药的相关性。方法收集上海市4所教学医院临床分离的鲍曼不动杆菌67株,采用琼脂稀释法测定其对常用抗菌药物的最低抑菌浓度。扩增所有临床株的7种PBP基因并测序。比较该菌氨苄西林-舒巴坦敏感组与耐药组之间核苷酸序列差异。结果临床分离鲍曼不动杆菌对常用抗菌药物耐药率高,对氨苄西林-舒巴坦耐药率为67.6%。测序结果显示敏感株及耐药株间未发现PBP的氨基酸变异。结论临床分离鲍曼不动杆菌对氨苄西林-舒巴坦耐药率较高。其耐药机制与PBP变异无相关性。

铜绿假单胞菌对β-内酰胺类抗生素耐药性主决定因素的研究

对 β-内酰胺类抗生素耐药的铜绿假单胞菌临床分离株的耐药机理进行了研究 ,内容包括 β-内酰胺酶的表达、细胞外膜通透性、主动外排和青霉素结合蛋白的改变等 ,重点研究了 2株对头孢他啶耐药且其MIC相似的临床分离铜绿假单胞菌 P.a.18SH和 P.a.143811。在这 2株菌中没有发现主动外排现象引起的细菌对 β-内酰胺类抗生素耐药 ,其中 ,P.a.18SH对头孢他啶的耐药性可由其低的细胞外膜通透性和高活性Class C类 β-内酰胺酶的表达来解释。P.a.143811有相当高的外膜通透性 ,其产生的 β-内酰胺酶特点与 P.a.18SH相似 ,但表达水平及总活性比 P.a.18SH酶低 ,与敏感菌相似。通过进一步的研究发现 ,P.a.143811的耐药性可能由于其具有多个 PBP基因突变 ,导致多个 PBPs对 β-内酰胺抗生素的敏感性发生改变或过度表达 ,其中的几个低分子量 PBPs可能与 D,D-羧肽酶活性有关。这是第一次在耐药的铜绿假单胞菌临床分离菌中报道 PBPs的过度表达。提示铜绿假单胞菌对β-内酰胺类抗生素的耐药性具有多样性 ,在新药研制和临床使用抗菌药物时应注意这些耐药特点。

肺炎链球菌β-内酰胺类抗生素最小抑菌质量浓度与青霉素结合蛋白1A和2B变异的关系

目的探讨肺炎链球菌(Sp)β-内酰胺类抗生素最小抑菌质量浓度(MIC)与青霉素结合蛋白(PBP)1A和2B变异的关系。方法对55株Sp用E-test法进行7种β-内酰胺类抗生素进行药敏试验,并提取每株Sp的DNA,分别对其青霉素结合蛋白基因(pbp)1a和pbp2b中编码青霉素结合区域(PBD)进行套式PCR扩增和直接测序,并用Clustalx软件进行序列比对,分析PBP1A和PBP2BPBD保守序列的氨基酸置换。结果青霉素敏感株4株中发现PBP2B保守序列SSN后苏氨酸(Thr)445→丙氨酸(Ala),Thr451→Ala和谷氨酸(Glu)481→甘氨酸(Gly)置换,其余6株PSSP未发现PBP1A和PBP2B保守序列氨基酸置换。4株青霉素中介株(PISP)(MIC0.19～0.38mg/L)PBP2BThr445→Ala,Thr451→Ala和Glu481→Gly置换,其中1株发现PBP2B保守序列SVVK后第431-432位点处脯氨酸(Pro)的插入,余3株存在谷氨酰胺(Gln)432→亮氨酸(Leu)置换。另16株PISP(MIC0.5～1.0mg/L)在此基础上出现PBP1ASRN后Pro432→Thr,STMK中Thr371→丝氨酸(Ser)/Ala和KTG附近的短镶嵌序列Thr574→天冬氨酸(ASn)Ser575→Thr,Gln576→Gly,苯丙氨酸(Phe)577→酪氨酸(Tyr)置换,且后二种变异存在于所有青霉素和头孢类中介和耐药株中。20/25株青霉素耐药株存在PBP2B保守序列KTG附近Ala624→Gly,包含Ala624→GlySp组青霉素、头孢呋新、阿莫西林等抗生素平均MIC值明显高于不包含这一置换的Sp组。在青霉素MIC≥0.5mg/L的菌株中均同时存在PBP1A和PBP2B的变异。结论β-内酰胺类抗生素对肺炎链球菌临床分离株MIC值与PBP1A和PBP2B编码青霉素结合活性区域的保守序列中或附近的氨基酸置换有关。

MRSA-PBP2a转肽酶区的原核表达及鉴定

为了对编码耐甲氧西林金黄色葡萄球菌(MRSA)青霉素结合蛋白2a(PBP2a)的转肽酶区(TPase)原核表达并进行Western blot鉴定。通过PCR方法由MRSA基因组中扩增转肽酶区基因片段,并构建pGEX-6p-1-TPase重组质粒,经酶切鉴定、测序正确后,转化BL-21,用IPTG进行诱导表达,并对表达的蛋白进行Western blot鉴定。结果表明,构建的pGEX-6p-1-TPase原核表达载体可表达PBP2a的转肽酶区蛋白,为其进一步的研究和应用奠定了基础。

新型青霉素结合蛋白基因(Bt-pbp2)的克隆、表达及其在青霉素残留检测中的应用

从苏云金芽胞杆菌中克隆到一种新型的青霉素结合蛋白基因Bt-pbp2,并在大肠杆菌中表达该蛋白,通过微量热泳动仪(MST)证实该蛋白与青霉素G有特异相互作用,其Kd值为10.36 nmol/L,利用该蛋白与青霉素G特异性相互作用,设计了竞争性酶联法检测牛奶中青霉素G残留的方法。研究表明,该方法当青霉素G浓度在4~256μg/L之间时,浓度与吸光度有线性关系,其添加回收率在93.4%±5.24%以上。研究表明,Bt-PBP2蛋白可以用于检测牛奶中青霉素残留,为进一步开发快速、高效青霉素残留检测试纸条设计奠定了基础。

抗MRSA-PBP2a鸡卵黄抗体的制备及乳胶凝集检测法的建立

制备抗耐甲氧西林金黄色葡萄球菌青霉素结合蛋白2a(MRSA-PBP2a)抗原的鸡卵黄免疫球蛋白(IgY),建立检测MRSA的乳胶凝集方法。采用体外诱导的方法制备PBP2a蛋白,胸部肌肉多点注射方式免疫6只海蓝蛋鸡,水稀释法提取IgY,BCA法测定蛋白含量,Western blotting进行特异性分析,用提取的IgY抗体致敏聚苯乙烯乳胶,建立检测PBP2a的乳胶凝集方法。成功诱导并制备获得纯化的PBP2a蛋白,首次免疫后1月每枚鸡蛋提纯后可获得约48 mg IgY抗体,Western blotting结果显示IgY抗体能有效识别纯化的PBP2a蛋白;成功建立检测PBP2a的乳胶凝集法,敏感性达1 mg/L。抗MRSA-PBP2a鸡卵黄抗体具有较高的敏感性和特异性,基于其建立的乳胶凝集检测方法具有较好的灵敏性。

β-内酰胺耐药粪肠球菌的低亲和力青霉素结合蛋白检测与多位点序列分型

目的检测临床分离粪肠球菌的耐药性、低亲和力青霉素结合蛋白pbp4基因和多位点序列分型(MLST)情况。方法收集临床分离的粪肠球菌78株,使用自动化仪器检测其耐药性;采用PCR扩增及基因测序的方法检测TEM基因和pbp4基因突变的突变情况;应用MLST对分离菌株进行进行多位点序列(MLST)分型。结果78株粪肠球菌对环丙沙星、左氧氟沙星、利福平、红霉素、四环素以及高浓度庆大霉素的耐药率较高,对青霉素和氨苄青霉素的耐药率为10.3%,未发现对呋喃妥因、万古霉素、替考拉宁和利奈唑胺耐药的菌株;78株粪肠球菌中有8株扩增出TEM基因,全部对青霉素和氨苄青霉素耐药,阳性率为10.3%;78株粪肠球菌共分为16个序列型,其中ST179型和ST16型最多,分别有21株和20株,占26.9%和25.6%,其余依次为ST6型8株(10.3%),ST4型7株(9.0%),ST585型6株(7.7%),ST480型4株(5.1%),ST28型3株(3.8%),其余各ST型只检出1株;分析ST型别与耐药性的关系显示相同ST型别的粪肠球菌具有类似的耐药谱。结论粪肠球菌对β-内酰胺类抗菌药物的耐药机制主要是由于产生由TEM基因介导的β-内酰胺酶所致,与pbp4基因的突变没有必然联系;粪肠球菌分离菌株主要以CC16(包含ST16和ST179)克隆株为主且耐药情况严重,需要针对其特点指导临床用药并加强院内感染监控。

沙颍河铅污染对儿童GH-IGF-1轴和体格发育的影响

目的：探讨沙颍河铅污染现状及其对儿童生长激素-胰岛素样生长因子-1（ GH-IGF-1）轴和体格发育的影响。方法：随机选择淮河沙颍河流域S县两个村庄作为调查点（依距河岸距离远近分别定为对照区和污染区）；原子吸收分光光度法检测河水和调查点饮用水及土壤中的铅含量。整群抽取两村庄小学8～13岁在校学生作为研究对象，伏安极谱法测定儿童血清铅含量；ELISA法检测儿童血清胰岛素样生长因子-1（ IGF-1）、胰岛素样生长因子结合蛋白3（IGFBP3）、生长激素（GH）和生长激素结合蛋白（GHBP）水平；电子体重计、身高坐高计、皮褶厚度计及Gulick卷尺分别测量体重、身高、皮褶厚度和胸围。结果：河水3个采样断面铅浓度均超过国家地表水水质标准Ⅴ级。污染区饮用水及土壤铅含量均高于对照区（ t＝2．663和2．300，P＜0．05）。污染区儿童血清铅含量高于对照区儿童（t＝3．227，P＝0．002）。污染区男孩身高、体重、皮褶厚度、胸围与对照区比较差异均无统计学意义（P均＞0．05）。两区女孩身高、体重和胸围差异均无统计学意义（P均＞0．05），但污染区女孩皮褶厚度高于对照区（t＝3．036，P＝0．003）。结论：沙颍河流域的饮用水中铅含量明显升高，污染区儿童血清GH-IGF-1轴相关因子水平受到影响。

胰岛素样生长因子结合蛋白-2与肺癌关系的研究进展

胰岛素样生长因子结合蛋白-2（Insulin like growth factor binding protein -2，IGFBP-2）作为肺癌高敏感的生物标记物，在肺癌的发生、发展及治疗中扮演重要的角色。研究显示其通过激活IGF1R及整合素介导的信号转导通路促进肿瘤的进展；且目前发现其在肺癌的靶向治疗中也起着重要的作用，有望成为肺癌治疗的新靶点，因此本文就IGFBP-2与肺癌的关系进行总结及综述。

pUC19-pbp2b重组质粒转化对肺炎链球菌感受态菌株耐药性的影响

目的探讨pUC19-pbp2b重组质粒转化对肺炎链球菌(SP)感受态菌株耐药性的影响。方法收集13株对青霉素不敏感的SP菌株,其中8株青霉素结合蛋白(PBPs)编码基因pbp2b未突变,5株pbp2b基因突变,制备SP感受态。化学合成含SSN保守区的pbp2b基因片段,构建pUC19-pbp2b重组质粒,将重组质粒转化感受态菌株。测定青霉素、头孢呋辛、头孢噻肟、头孢曲松和头孢吡肟5种β-内酰胺酶类抗生素(BLA)对转化前后SP感受态菌株的最小抑菌浓度(MIC)。结果 pbp2b基因扩增产物可见约300 bp的特异条带,13株SP菌株均能形成感受态。与转化前菌株比较,5种抗生素对转化后菌株的MIC均降低(P<0.05)。5种抗生素对5株转化后的pbp2b基因突变菌株的MIC均降低(P<0.05)。结论外源重组质粒转化SP感受态可以协助减缓SP耐药性的进展。

青霉素结合蛋白的重组表达及其在β-内酰胺类抗生素检测中的应用

目的获得纯化的重组青霉素结合蛋白(penicillin binding proteins,PBPs),研究其在β-内酰胺类抗生素检测中的应用。方法以来源于肺炎链球菌Streptococcus pneumoniae R6的PBP2x蛋白为对照,以PBP1a蛋白作为目标受体,研究其与β-内酰胺类抗生素的亲和作用。结果经纯化后的重组蛋白PBP2x和PBP1a检测头孢噻呋、青霉素G、氨苄青霉素、喷沙西林、阿莫西林的半抑制浓度(inhibitory concentration,IC_(50))都在7.02 ng/mL以下,明确了PBP1a和PBP2x具有β-内酰胺类抗生素结合能力。结论该研究为开发新的基于PBPs蛋白检测β-内酰胺类抗生素的免疫学方法奠定了基础。

高表达GFP-PBP1b融合蛋白的猪链球菌菌株的构建及PBP1b蛋白细胞定位的研究

为鉴定猪链球菌(Streptococcus suis)A型青霉素结合蛋白PBP1b在S.suis中的细胞定位,本研究经PCR扩增S.suis pbp1b基因融合位点上下游序列UP和DN、强启动子Peno基因片段及绿色荧光蛋白(GFP)gfp基因片段,再通过重叠延伸PCR扩增构建融合片段UP-Peno-GFP-DN。利用同源重组的方法将UP-Peno-GFP-DN转化含反向筛选标记的PSS-pbp1b中间菌株,经含7%蔗糖的TSAS平板筛选,挑单菌落进行PCR及测序鉴定。PCR及测序鉴定结果显示,获得的重组菌株中Peno-gfp片段替换了PSS-pbp1b中的PSS片段,表明融合强启动子Peno、GFP及PBP1b(GFP-PBP1b)的重组菌株P-GFP-pbp1b正确构建。以S.suis 05ZYH33株和本实验室前期构建的GFP-pbp1b为对照,培养P-GFP-pbp1b菌株并测定OD600nm值,绘制各菌株的生长曲线;采用western blot检测P-GFP-pbp1b菌株中GFP-PBP1b融合蛋白的表达水平,并与GFP-pbp1b菌株进行比较;利用Alexa Fluor 633-WGA染色,经超高分辨显微镜观察GFP-pbp1b和P-GFP-pbp1b菌株形态及GFP-PBP1b融合蛋白在S.suis细胞中的定位。生长曲线结果显示,S.suis融合菌株GFP-pbp1b和P-GFP-pbp1b均正常生长;western blot结果显示,GFP-pbp1b和P-GFP-pbp1b菌株均能够表达GFP-PBP1b融合蛋白,但强启动子驱动的P-GFP-pbp1b菌株中GFP-PBP1b蛋白表达量较GFP-pbp1b菌株提高了6倍(P<0.01);超高分辨显微镜观察结果显示,GFP-pbp1b和P-GFP-pbp1b菌株形态均正常,GFP-pbp1b菌株中GFP荧光较弱,难以定位GFP-PBP1b,而P-GFP-pbp1b菌株中GFP荧光较强,能够明显观察到融合蛋白GFP-PBP1b定位在S.suis的细胞横隔和两极。本研究通过构建高表达GFP-PBP1b融合蛋白的P-GFP-pbp1b菌株首次观察到PBP1b在S.suis中的细胞定位,为进一步研究PBP1b在S.suis细胞壁肽聚糖合成中的作用奠定了基础。

Long non-coding RNA DPP10-AS1 represses the proliferation and invasiveness of glioblastoma by regulating miR-24-3p/CHD5 signaling pathway

This investigation aimed to unveil new prospective diagnosis-related biomarkers together with treatment targets against glioblastoma.Methods:The expression levels of long non-coding RNA(lncRNA)DPP10-AS1 were assessed using real-time quantitative polymerase chain reaction(RT-qPCR)within both the patient tissue specimens and glioblastoma cell lines.The relationship between lncRNA DPP10-AS1 expression in glioblastoma and patient prognosis was investigated.Cell Counting Kit-8(CCK-8),transwell,and clonogenic experiments were utilized to assess tumor cells’proliferation,invasiveness,and migratory potentials after lncRNA DPP10-AS1 expression was up or down-regulated.Using an online bioinformatics prediction tool,the intracellular localization of lncRNA DPP10-AS1 and its target miRNA were predicted,and RNA-FISH verified results.A dual-luciferase reporter experiment validated the relationship across miR-24-3p together with lncRNA DPP10-AS1.MiR-24-3p expression within glioblastoma was identified through RT-qPCR,and potential link across miR-24-3p and lncRNA DPP10-AS1 was assessed using Pearson correlation analysis.Moreover,influence from lncRNA DPP10-AS1/miR-24-3p axis upon glioblastoma cell progression was assessed in vivo via a subcutaneous xenograft tumor model.Results:The expression of lncRNA DPP10-AS1 was notably reduced in both surgical specimens of glioblastoma and the equivalent cell lines.Low level of lncRNA DPP10-AS1 in glioblastoma is following poor prognosis.The downregulation of lncRNA DPP10-AS1 in glioblastoma cells resulted in enhanced cellular proliferation,migration,and invasion capabilities,accompanied by downregulated E-cadherin and upregulated vimentin and N-cadherin.Additionally,the observed upregulation of lncRNA DPP10-AS1 demonstrated a substantial inhibitory function upon proliferation,invasion,and migratory capabilities of LN229 cells.Subcellular localization disclosed that lncRNA DPP10-AS1 had a binding site that interacted with miR-24-3p.Upregulated miR-24-3p was detected in glioblastomas,displaying an inverse correlation with lncRNA DPP10-AS1 expression.MiR-24-3p downstream target has been determined as chromodomain helicase DNA binding protein 5(CHD5).LncRNA DPP10-AS1 affected the invasion and proliferation of glioblastoma by controlling the miR-24-3p/CHD5 axis.Conclusion:The present study demonstrated that lncRNA DPP10-AS1 can inhibit the invasive,migratory,and proliferative properties of glioblastoma by regulating the miR-24-3p/CHD5 signaling pathway.Consequently,lncRNA DPP10-AS1 has potential as a tumor suppressor and might be utilized for accurate diagnosis and targeted treatments of glioblastomas.