Diagnostic value of methylated branched chain amino acid transaminase 1/IKAROS family zinc finger 1 for colorectal cancer

BACKGROUND The diagnostic value of combined methylated branched chain amino acid transaminase 1(BCAT1)/IKAROS family zinc finger 1(IKZF1)in plasma for colorectal cancer(CRC)has been explored since 2015.Recently,several related studies have published their results and showed its diagnostic efficacy.AIM To analyze the diagnostic value of methylated BCAT1/IKZF1 in plasma for screening and postoperative follow-up of CRC.METHODS The candidate studies were identified by searching the PubMed,Embase,Cochrane Library,CNKI,and Wanfang databases from May 31,2003 to June 1,2023.Sensitivity,specificity,and diagnostic accuracy were calculated by merging ratios or means.RESULTS Twelve eligible studies were included in the analysis,involving 6561 participants.The sensitivity of methylated BCAT1/IKZF1 in plasma for CRC diagnosis was 60%[95%confidence interval(CI)53-67]and specificity was 92%(95%CI:90-94).The positive and negative likelihood ratios were 8.0(95%CI:5.8-11.0)and 0.43(95%CI:0.36-0.52),respectively.Diagnostic odds ratio was 19(95%CI:11-30)and area under the curve was 0.88(95%CI:0.85-0.91).The sensitivity and specificity for CRC screening were 64%(95%CI:59-69)and 92%(95%CI:91-93),respectively.The sensitivity and specificity for recurrence detection during follow-up were 54%CONCLUSION The detection of methylated BCAT1/IKZF1 in plasma,as a non-invasive detection method of circulating tumor DNA,has potential CRC diagnosis,but the clinical application prospect needs to be further explored.

Intracellular accumulation of tau inhibits autophagosome formation by activating TIA1-amino acid-mTORC1 signaling

Background:Autophagy dysfunction plays a crucial role in tau accumulation and neurodegeneration in Alzheimer’s disease(AD).This study aimed to investigate whether and how the accumulating tau may in turn affect autophagy.Methods:The primary hippocampal neurons,N2a and HEK293T cells with tau overexpression were respectively starved and treated with vinblastine to study the effects of tau on the initiating steps of autophagy,which was analysed by Student’s two-tailed t-test.The rapamycin and concanamycin A were employed to inhibit the mammalian target of rapamycin kinase complex 1(mTORC1)activity and the vacuolar H+-ATPase(v-ATPase)activity,respectively,which were analysed by One-way ANOVA with post hoc tests.The Western blotting,co-immunoprecipitation and immunofuorescence staining were conducted to gain insight into the mechanisms underlying the tau effects of mTORC1 signaling alterations,as analysed by Student’s two-tailed t-test or One-way ANOVA with post hoc tests.The autophagosome formation was detected by immunofuorescence staining and transmission electron microscopy.The amino acids(AA)levels were detected by high performance liquid chromatography(HPLC).Results:We observed that overexpressing human full-length wild-type tau to mimic AD-like tau accumulation induced autophagy deficits.Further studies revealed that the increased tau could bind to the prion-related domain of T cell intracellular antigen 1(PRD-TIA1)and this association significantly increased the intercellular level of amino acids(Leucine,P=0.0038;Glutamic acid,P=0.0348;Alanine,P=0.0037;Glycine,P=0.0104),with concordant upregulation of mTORC1 activity[phosphorylated eukaryotic translation initiation factor 4E-binding protein 1(p-4EBP1),P<0.0001;phosphorylated 70 kD ribosomal protein S6 kinase 1(p-p70S6K1),P=0.0001,phosphorylated unc-51-like autophagyactivating kinase 1(p-ULK1),P=0.0015]and inhibition of autophagosome formation[microtubuleassociated protein light chain 3 II(LC3 II),P=0.0073;LC3 puncta,P<0.0001].As expected,this tau-induced deficit of autophagosome formation in turn aggravated tau accumulation.Importantly,we also found that blocking TIA1 and tau interaction by overexpressing PRD-TIA1,downregulating the endogenous TIA1 expression by shRNA,or downregulating tau protein level by a small proteolysis targeting chimera(PROTAC)could remarkably attenuate tau-induced autophagy impairment.Conclusions:Our findings reveal that AD-like tau accumulation inhibits autophagosome formation and induces autophagy deficits by activating the TIA1/amino acid/mTORC1 pathway,and thus this work reveals new insight into tau-associated neurodegeneration and provides evidence supporting the use of new therapeutic targets for AD treat-ment and that of related tauopathies.

支链氨基酸转氨酶1在食管鳞癌中的表达及其临床意义

目的探讨食管鳞癌(ESCC)患者癌组织中支链氨基酸转氨酶1(BCAT1)的表达及临床意义。方法采用qRT-PCR和Western blot技术检测食管鳞癌细胞系中BCAT1基因的表达水平,筛选出合适的食管癌细胞,作为后续研究。敲低和过表达BCAT1,采用Western blot检测ESCC细胞中BCAT1的蛋白表达水平。CCK-8活力测定、克隆形成实验、划痕实验、Transwell检测ESCC细胞增殖、迁移和侵袭等细胞表型的变化。结果qRT-PCR和Western blot结果显示,与正常细胞相比,BCAT1在ESCC中的相对表达量降低,尤其是KYSE150和Eca109细胞更为明显,因此选择这两株细胞进行研究。CCK-8细胞增殖实验结果显示,细胞在转染BCAT1 siRNA 48 h后,其增殖率明显高于对照组;而过表达BCAT1之后,效果则相反。克隆形成实验结果表明,BCAT1的敲低显著促进ESCC细胞的克隆形成,而BCAT1的过表达显著抑制ESCC细胞的克隆形成。细胞划痕实验和Transwell实验结果表明,与Control siRNA组相比,BCAT1 siRNA组ESCC细胞的迁移和侵袭明显升高;而过表达组中ESCC细胞的迁移和侵袭明显受到抑制。结论BCAT1在ESCC中低表达,BCAT1低表达显著促进ESCC细胞增殖、迁移和侵袭。

L型氨基酸转运蛋白1的表达对非霍奇金淋巴瘤临床病理特征和预后的影响

目的:检测非霍奇金淋巴瘤(NHL)组织中L型氨基酸转运蛋白1(LAT1)的表达,分析LAT1对患者临床病理特征和预后的影响。方法:收集2017年1月至2019年4月在本院接受治疗的NHL患者92例,免疫组织化学检测NHL组织中LAT1的表达,比较不同病理特征(包括性别、Ann Arbor分期、结外浸润、Ki-67)患者组间LAT1的表达差异,单因素和多因素Cox回归分析影响患者死亡的危险因素,受试者工作曲线(ROC)检测NHL组织中LAT1阳性细胞百分比对患者死亡的预测价值,分析LAT1阳性细胞百分比对患者生存率的影响。结果:LAT1在NHL组织中呈阳性表达,Ann Arbor分期III期和IV期组LAT1高表达率高于I期组,结外浸润组LAT1高表达率高于无结外浸润组,Ki-67阳性表达组LAT1高表达率高于阴性表达组,比较差异均有统计学意义(均P<0.05)。LAT1高表达组治疗3个疗程后的缓解率为70.7%,低于低表达组的91.2%,比较差异有统计学意义(P<0.05)。Ann Arbor分期III期、IV期、结外浸润、Ki-67阳性表达和LAT1表达增加(即LAT1阳性细胞比例评分≥2)为患者死亡的危险因素。LAT1阳性细胞百分比预测NHL死亡的截断值为45.6%,曲线下面积为0.905(95%CI:0.897-0.924)。LAT1高水平组(LAT1阳性细胞百分比≥45.6%)3年生存率为50.00%,低于LAT1低水平组的78.26%(P<0.05)。结论:LAT1在NHL组织中表达水平增加,影响患者的肿瘤分期和结外浸润,是患者死亡的危险因素。

BCAT1抑制剂BAY-069的合成工艺优化

BAY-069是目前体外活性最强的支链氨基酸转氨酶1(BCAT1)抑制剂,但其报道的合成路线存在原料成本较高、总收率极低和中间体结构表征不充分等缺点。本研究基于已有合成路线,重点对其合成工艺中的Ullmann偶联反应进行了系统优化。以1-硝基萘(1)为起始原料,经过7步反应和手性色谱柱手性拆分合成目标化合物BAY-069。所有中间体和目标化合物均经1 H NMR,13 C NMR和HR-MS表征。以Ullmann偶联反应为主要优化步骤的路线,其优化后的总收率为11.0%(3b→(±)-BAY-069),是原总收率1.6%(3a→(±)-BAY-069)的6.9倍。

BCAT1作为胰腺导管腺癌潜在诊断标志物的临床应用价值研究

目的 本研究拟验证前期研究发现的bcat1基因表达产物支链氨基酸转氨酶1(BCAT1)作为胰腺导管腺癌潜在血清学诊断标志物的临床应用价值。方法 收集临床PDAC患者血清样本作为实验组,收集胃癌、肝癌、结直肠癌、慢性胰腺炎患者及健康人群血清样本作为对照,采用酶联免疫吸附实验(ELISA)检测血清样本BCAT1浓度,验证其作为标志物的临床诊断价值。结果 ELISA结果显示PDAC组患者血清BCAT1浓度显著高于健康对照组,差异有统计学意义(P<0.05,U=1 206)。PDAC组患者血清BCAT1浓度高于慢性胰腺炎组,差异有统计学意义(P<0.05,H=33.80);与其他消化道肿瘤相比,高于肝癌组和结直肠癌组,差异有统计学意义(P<0.05,H=33.80),与胃癌组差异无统计学意义(P>0.05,H=33.80)。BCAT1与CA19-9的相关性较好,且差异有统计学意义(P<0.05,R^(2)=0.080 52),与CEA(R^(2)=2.265e-005)、CA125(R^(2)=0.025 88)和CA72-4(R^(2)=0.007 7)相关性较低,差异无统计学意义(P>0.05);BCAT1诊断PDAC的AUC优于CA72-4,与CA125和CEA相当,劣于CA19-9;BCAT1 cut off值为1.556ng/mL,敏感度为64.1%,特异度为80%。BCAT1在PDAC早中期患者血清浓度中位数为0.283 ng/mL,晚期患者升高为0.482 ng/mL,差异有统计学意义(P<0.05,U=1029);在肿瘤≥40 mm(U=641)、中低分化(U=435)、胰头部位(H=2.767)均表现为表达水平升高,差异无统计学意义(P均>0.05)。动态观测的BCAT1浓度在第0天和1~30天(U=44)、31~60天和61~90天(U=36)浓度差异有统计学意义(P均<0.05)。结论 BCAT1作为潜在的血清学标志物,对于PDAC的鉴别诊断、肿瘤分期、疾病进展判断具有参考价值,是目前现有的PDAC血清标志物的有益补充。

Expression of L amino acid transport system 1 and analysis of iodine-123-methyltyrosine tumor uptake in a pancreatic xenotransplantation model using fused high-resolution-micro-SPECT-MRI

BACKGROUND:The specificity in discriminating pancreatitis is limited in the positron emission tomography(PET)using Fluorine-18-fluorodeoxyglucose.Furthermore,PET is not widely available compared to the single photon emission computed tomography(SPECT).Since amino acids play a minor role in metabolism of inflammatory cells,the potential of the SPECT tracer,3-[ 123 I]iodo-L-α-methyltyrosine(123I-IMT),for detecting pancreatic cancer was examined in xenotransplantation models of human pancreatic carcinoma in mice. METHODS: 123 I-IMT was injected to eight mice inoculated with subcutaneous or orthotopic pancreatic tumors.Fused high-resolution-micro-SPECT(Hi-SPECT)and magnetic resonance imaging were performed.The gene expression level of L amino acid transport-system 1(LAT1)was analyzed and correlated with tumor uptake of 123 I-IMT. RESULTS:A high uptake of 123 I-IMT was detected in all tumor-bearing mice.The median tumor-to-background ratio (T/B)was 12.1(2.0-13.2)for orthotopic and 8.4(1.8-11.1)for subcutaneous xenotransplantation,respectively.Accordingly, the LAT1 expression in transplanted Colo357 cells was increased compared to non-malignant controls.CONCLUSIONS:Our mouse model could show a high 123 I-IMT uptake in pancreatic cancer.Fused MRI scans facilitate precise evaluation of uptake in the specific regions of interest.Further studies are required to confirm these findings in tumors derived from other human pancreatic cancer cells.Since amino acids play a minor role in the metabolism of inflammatory cells,the potential for application of 123 I-IMT to distinguish pancreatic tumor from inflammatory pancreatitis warrants further investigation.

Simultaneous Determination of Dopamine and Uric Acid at 2-Amino-5-mercapto-[1, 3, 4]triazole Self-assembled Monolayers Gold Electrode

A newly synthesized reagent 2-amino-5-mercapto-[1, 3, 4]triazole (MATZ) has been usedto fabricate self-assembled monolayers (SAMs) on gold electrode for the first time. The SAMselectrode was characterized by electrochemical methods and scanning electronic microscopy (SEM),the SAMs electrode can be used to determinate dopamine (DA) and uric acid (UA) simultaneouslywith a detection limit of 8×10-7 mol/L for DA and 1×10-6 mol/L for UA respectively. The SAMscan also be used to detect the contents of DA and UA in synthetic urine sample with satisfactoryresults.

HIV-1 Env gp120 C2V5 Potential N-Linked Glycosylation Site(s) (PNGs) Variations and Amino Acid Length Polymorphisms among Infected Family Members

Objective: To ascertain the role of HIV-1 gp120 env PNGs variations and sequence length polymorphism following transmission events as possible supporting forensic evidence to determine directionality of HIV transmission. Method: An observational study of HIV-1 infected family members, where median and range values of the amino acid lengths and PNGs for the genotyped C2V5 region were calculated. Wilcoxon rank-sum test was used to determine differences in these parameters between different family members. Results: For heterosexual transmission, two mothers had longer C3 sequences relative to that of their spouses;p=0.006 and=0.025 whilst the opposite was observed for one mother, p = 0.028. No clear trends were observed for PNGs. Index children had longer C2V5 amino acid sequences compared to their mothers p = 0.013, 0.040, 0.043 for families 205, 375, 567 respectively. Second siblings “V4 and V5 sequences were generally shorter relative to the maternal ones p = 0.039 and 0.028, respectively. Adults had longer V3 amino acid sequences compared to children;p = 0.018. Similar trends were also observed regarding PNGs within the entire C2V5 region, C3 and V4 sub-regions;p= 0.0025, 0.005 and 0.008, respectively. First siblings’ C2V5 and C3 sequence lengths were significantly longer relative to those of the second siblings;p = 0.005 and 0.007, respectively. Conclusion: Our results are suggestive that HIV-1 env C2V5 amino acid length polymorphism and PNGs tend to increase with age and HIV disease progression. Though sensitive and should be cautiously handled, it is tempting to propose the direc-tionality of the HIV transmission events with respect to C3 sequence length polymorphisms. Correlating HIV-1 env C2V5 amino acid length polymorphism and age of infection may be the first step towards a possible valuable piece of forensic evidence which may be useful in criminalisation of willful HIV infections. However, bigger studies are war-ranted to substantiate the authenticity of this potentially useful application.

Synthetic Studies on 1-Amino-1-Cyclopropane-Carboxylic Acid( Ⅰ )——The Cyclopropanation via Addition-Elimination Reactions

Various addition-elimination approaches have been explored for diastereoselective construction of 1-amino- 1-cyclopropane-carboxylic acid (ACPC) derivatives, and the desired product was obtained from a reaction of cyclo(NAc-L-Val-NAc-Gly) and methyl α-bro-moacrylate under protonic solvent.

Swelling Properties of New Hydrogels Based on the Dimethyl Amino Ethyl Acrylate Methyl Chloride Quaternary Salt with Acrylic Acid and 2-Methylene Butane-1,4-Dioic Acid Monomers in Aqueous Solutions

Hydrogels of dimethylaminoethyl acrylate methyl chloride quaternary salt (Q9) have been synthesized with different monomer ratio by copolymerization of this poorly studied monomer either with acrylic acid or with 2-methylene bu-tane-1,4-dioic acid. Hydrogel swelling was measured as a function of the composition of the hydrogel and of the crosslinking agent ratio. High values of swelling have been obtained at very high crosslinking values (【14 wt %) and the equilibrium swelling was reached at very low time (less than 15 minutes). The swelling isotherms consisted of a steep initial portion and then levelled off as asymptotically to the equilibrium swelling limit. The experimental data suggest clearly that the swelling process obeys second-order kinetics. According to this, the kinetics rate constant and the equilibrium water content were determined at different comonomer composition and crosslinker concentration. The calculated kinetic constants ranged from 0.48 to 3.76 &#215;10-2 min-1 for poly (acrylic acid-co-Q9) hydrogels and from 0.68 to 4.0 &#215;10-2 min-1 for poly (2-methylene butane-1,4-dioic acid-co-Q9) hydrogels depending on the hydrogels composition. The diffusion process was evaluated for each hydrogel showing a non-Fickian type diffusion. In all cases was observed a considerable increase in diffusion coefficient as Q9 content increases.

LAT1表达水平与非肌层浸润性膀胱癌患者术后复发风险的相关性研究

目的:探讨L型氨基酸转运蛋白1(L-type amino acid transporter 1,LAT)表达水平与非肌层浸润性膀胱癌患者术后复发风险的相关性。方法:选取2021年2月至2022年2月于重庆医科大学附属永川医院接受手术治疗的非肌层浸润性膀胱癌患者108例作为研究对象,采用反转录酶聚合酶链反应测定膀胱癌组织(取自肿瘤所在部位区域)和癌旁组织(取自邻近正常区域组织)LAT1表达含量,对比膀胱癌组织和癌旁组织LAT1表达水平。同时根据膀胱癌组织LAT1表达含量的二分位数将所有患者分为高表达组和低表达组,对比2组临床病理参数。随访观察12个月观察2组术后复发情况,采用Kaplan-Meier曲线分析对比2组术后复发风险,使用多变量Cox比例风险回归模型确定术后复发的影响因素。结果:膀胱癌组织LAT1表达水平(1.80±0.35)较配对的癌旁组织LAT1表达水平(1.05±0.17)高(P<0.05);LAT1高表达组吸烟史、临床分期T_1占比较LAT1低表达组高(P<0.05);108例膀胱肿瘤患者术后的平均随访时间为(10.84±1.94)个月,其中33例复发,复发率为30.56%。KaplanMeier曲线显示,LAT1高表达组患者总体复发率较LAT1低表达组高(log-rank χ^(2)=4.382,P=0.036);多因素Cox回归分析显示,吸烟史(HR=6.539,95%CI=2.439~17.531)、临床分期为T_1期(HR=3.658,95%CI=1.808~7.398)、LAT1高表达(HR=3.425,95%CI=1.631~7.191)为非肌层浸润性膀胱癌患者术后复发的危险因素(P<0.05)。结论:LAT1在膀胱癌组织中表达水平高,高LAT1表达水平可能与膀胱癌患者术后复发风险增加有关。

补肾益气活血方对FGR大鼠小肠上LAT1表达的影响

目的观察补肾益气活血方对宫内生长受限(fetal growth restriction,FGR)大鼠小肠上氨基酸转运蛋白LAT1表达的影响,探讨该方治疗胎儿宫内生长受限的可能机制。方法应用被动吸烟法构建Wistar大鼠FGR模型,将35只孕鼠随机分为空白组、模型组、中药组、西药组及中西药结合组,其中5只孕鼠未获得胎鼠,最终30只孕鼠入组。采用Realtime RT-PCR法、Western Blot法检测胎鼠及孕鼠小肠上氨基酸转运蛋白LAT1(SLC7A5)及其重链4F2hc(SLC3A2)的mRNA及蛋白表达,并比较其表达差异。结果FGR模型组孕鼠小肠上氨基酸转运蛋白LAT1及其对应mRNA SLC7A5表达上调,经补肾益气活血方和(或)精氨酸治疗后出现不同程度的表达下调,且各治疗组胎鼠体重均高于FGR模型组。结论孕鼠小肠上LAT1蛋白及mRNA表达下调可能与补肾益气活血方治疗宫内生长受限的作用机制有关。

敲除TSP1通过氨基酸和糖代谢通路对阿霉素所致心肌损伤的作用

目的利用代谢组学方法阐明敲除血小板反应蛋白1(TSP1)通过调节小分子化合物的代谢,减轻阿霉素(ADM)致心肌损伤。方法以24只野生型C57BL/6小鼠和24只TSP1基因敲除(TSP1^(-/-))小鼠为实验对象,分为4组:WM组(n=12)、TSP1^(-/-)组(n=12)和WM-ADM组(n=12)、TSP1^(-/-)-ADM组(n=12)。WM组和TSP1^(-/-)组小鼠腹腔注射生理盐水,WM-ADM组和TSP1^(-/-)-ADM组小鼠腹腔注射ADM以建立慢性心功能衰竭(CHF)模型。以血清生化[肌酸激酶(creatine kinase,CK)、肌酸激酶同工酶(creatine kinase isoenzymes,CK-MB)、乳酸脱氢酶(lactate dehydrogenase,LDH)]和心脏组织苏木精-伊红(hematoxylin-eosin,HE)染色为指标评价注射ADM后小鼠心肌损伤情况,以基于核磁共振(1HNMR)的代谢组学技术来研究4组小鼠血清中小分子代谢物的变化。结果血清生化和心脏组织HE染色显示,注射ADM后TSP1^(-/-)小鼠心脏组织损伤比野生小鼠明显减轻。代谢组学研究显示,敲除TSP1后明显影响小鼠体内的氨基酸代谢。野生型小鼠注射ADM后,血清亮氨酸、异亮氨酸、缬氨酸、乳酸、丙氨酸、乙酸和丙酮酸等变化明显;TSP1^(-/-)小鼠注射ADM后上述血清代谢物水平明显回调。结论本研究发现TSP1^(-/-)小鼠可能通过调节氨基酸和糖代谢来减弱ADM造成的心肌损伤。

支链氨基酸转移酶1在肿瘤发生与进展中的作用机制

支链氨基酸转移酶1(branched-chain amino acid transaminase 1,BCAT1)催化支链氨基酸(branched-chain amino acids,BCAA)和支链酮酸(branched-chain keto acids,BCKA)之间的转换反应,在维持二者稳态中发挥重要作用。近年来人们发现,BCAT1在多种恶性肿瘤中高表达,且与癌症的分期和预后关系密切,进一步研究证实,BCAT1能促进癌细胞的增殖、侵袭和转移,并揭示BCAT1在癌症发生发展中的部分作用机制:(1)不同肿瘤中BCAT1催化转氨基反应的方向不同,BCAT1既可催化BCAA分解为BCKA,也可催化BCKA合成BCAA,这两个方向都可能促进癌症的发生和发展;(2)BCAT1既能直接影响肿瘤细胞代谢来发挥相关作用,也能通过影响肿瘤微环境而产生促癌效应。总体而言,BCAT1通过催化BCAA的分解与合成反应,影响物质代谢、能量合成、信号通路、肿瘤免疫、表观遗传学和细胞周期等方面,进而促进癌症的发生与进展。本文就国内外BCAT1和BCAA的研究进展,聚焦BCAT1在肿瘤发生发展中的作用机制做一综述,为进一步探讨BCAT1在恶性肿瘤研究中的应用前景提供理论依据。

气相色谱法测定7-氨基-3-(丙烯-1-基)-3-头孢烯-4-羧酸中溶剂残留量

建立气相色谱法同时测定7-氨基-3-(丙烯-1-基)-3-头孢烯-4-羧酸中丙酮、四氢呋喃、甲醇和二氯甲烷溶剂残留量的方法。7-氨基-3-(丙烯-1-基)-3-头孢烯-4-羧酸样品使用0.1%氢氧化钠溶液进行超声溶解,使用HP-FFAP毛细管柱进行化合物的分离,氢离子火焰检测器进行测定,外标法定量。丙酮、甲醇、二氯甲烷和四氢呋喃均能获得基线分离,甲醇、丙酮、四氢呋喃和二氯甲烷的质量浓度分别在5.1~657.6 mg/L,2.1~677.1 mg/L,2.3~681.9 mg/L和2.4~728.0 mg/L范围内与其色谱峰面积具有良好线性关系,线性相关系数为0.9994~0.9999,甲醇、丙酮、四氢呋喃和二氯甲烷定量限分别为107.1、52.9、57.5、60.0 mg/kg。丙酮、甲醇、二氯甲烷和四氢呋喃测定结果的相对标准偏差均不大于2.56%(n=6),平均加标回收率为92.53%~109.96%。该方法适用于7-氨基-3-(丙烯-1-基)-3-头孢烯-4-羧酸中溶剂残留量的定性、定量分析。

SLC1A5协同TM4SF1通过mTOR信号通路调控食管鳞癌细胞迁移

目的探讨氨基酸转运载体溶质载体家族1成员5(SLC1A5)在食管鳞癌(ESCC)中的表达及其与临床病理特征的相关性,以及SLC1A5对ESCC细胞迁移的影响及潜在分子机制。方法采用TNM plot在线数据库分析SLC1A5基因在ESCC组织和正常组织中的表达情况。通过实时定量逆转录聚合酶链反应(qRT-PCR)法检测ESCC组织和癌旁组织中SLC1A5 mRNA表达情况;采用免疫组化(IHC)法检测SLC1A5蛋白表达情况,并分析其与患者临床病理资料的相关性。分别构建SLC1A5过表达(SLC1A5-OE组)、四跨膜蛋白超家族成员1过表达(TM4SF1-OE组)、SLC1A5和TM4SF1共同过表达的Eca109细胞。采用细胞增殖试验、Transwell实验检测Eca109细胞的增殖、迁移和侵袭能力。通过免疫共沉淀(IP)实验证实SLC1A5和TM4SF1的相互作用;采用蛋白质免疫印迹(WB)法检测哺乳动物雷帕霉素靶蛋白(mTOR)信号通路相关蛋白的表达水平。结果TNM plot数据库分析显示,ESCC组织中SLC1A5基因表达水平高于正常组织,差异有统计学意义(P<0.05)。ESCC组织中SLC1A5 mRNA表达高于成对的癌旁组织,差异有统计学意义(P<0.01)。IHC结果显示,SLC1A5蛋白在癌组织中高表达,并且与临床分期(P=0.036)、淋巴结转移(P=0.029)显著相关。细胞增殖实验结果显示,SLC1A5-OE组和对照细胞(Con组)增殖能力比较,差异无统计学意义(P>0.05)。Transwell实验结果显示,与Con组比较,SLC1A5-OE组细胞迁移及侵袭能力增强,差异有统计学意义(P<0.01)。IP结果表明,SLC1A5与TM4SF1存在相互作用。WB结果显示,相对于SLC1A5-OE组或TM4SF1-OE组,p-mTOR、p-S6蛋白表达水平在SLC1A5和TM4SF1共同过表达的细胞中最高。Transwell实验证实,共同过表达SLC1A5和TM4SF1的ESCC细胞迁移能力最强。结论ESCC中SLC1A5呈高表达,且与患者临床分期、淋巴结转移显著相关,SLC1A5可能通过与TM4SF1相互作用,激活mTOR信号通路,进而促进ESCC细胞迁移。

水稻氨基酸透性酶基因OsAAP14启动子克隆及时空表达特性分析

【目的】克隆水稻氨基酸透性酶基因OsAAP14的启动子序列并分析其时空表达特性,为解析氨基酸转运基因生物学功能及了解水稻对有机氮源的响应和氨基酸吸收利用提供理论依据。【方法】PCR扩增OsAAP14基因的启动子序列,并与p CAMBIA1391Z空载体质粒连接构建出启动子-GUS表达载体,并通过农杆菌介导侵染水稻中花11愈伤组织,获得OsAAP14基因的启动子-GUS转基因植株,通过对转基因植株不同组织部位进行GUS染色,并采用石蜡切片技术观察各组织细胞部位表达,经5种不同氨基酸处理后进行根部GUS染色,结合实时荧光定量PCR检测OsAAP14基因在GUS染色部位的相对表达量,最后综合分析该基因的时空表达特性。【结果】克隆获得OsAAP14基因启动子序列为1993 bp,与参考序列日本晴OsAAP14(LOC_Os04g56470)序列一致。该启动子序列含有MBS、P-box、ABRE、CGTCA-motif等激素或胁迫响应元件。从OsAAP14基因的启动子-GUS植株T0代中鉴定获得16个阳性转基因株系。T1代材料不同组织部位GUS染色及实时荧光定量PCR结果均显示,OsAAP14基因在水稻芽伸长的基部和叶片相对表达量较高,在根、叶鞘和穗也有一定表达,但在茎中的相对表达量最低。石蜡切片分析结果显示,OsAAP14基因在根部皮层薄壁细胞、叶片的叶肉细胞、穗的颖壳内部细胞有较高的表达。碱性氨基酸的组氨酸处理下根中的OsAAP14基因表达量随着处理时间的增加显著提高(P<0.05,下同),且赤霉素和脱落酸处理下,根中的OsAAP14基因相对表达量也显著提高。【结论】OsAAP14基因在水稻不同组织均有表达,正常情况(未处理)下在水稻基部和叶片中相对表达量较高,但外源氨基酸和激素处理时,在根中该基因被诱导表达上调,说明OsAAP14基因正常情况下可能主要参与调控水稻地上部分氨基酸的运输,但当外界氨基酸和激素含量增加时则参与调控水稻根部氨基酸的运输。

Estrogen affects neuropathic pain through upregulating N-methyl-D-aspartate acid receptor 1 expression in the dorsal root ganglion of rats

Estrogen affects the generation and transmission of neuropathic pain,but the specific regulatory mechanism is still unclear.Activation of the N-methyl-D-aspartate acid receptor 1（NMDAR1） plays an important role in the production and maintenance of hyperalgesia and allodynia.The present study was conducted to determine whether a relationship exists between estrogen and NMDAR1 in peripheral nerve pain.A chronic sciatic nerve constriction injury model of chronic neuropathic pain was established in rats.These rats were then subcutaneously injected with 17β-estradiol,the NMDAR1 antagonist D（-）-2-amino-5-phosphonopentanoic acid（AP-5）,or both once daily for 15 days.Compared with injured drug na？ve rats,rats with chronic sciatic nerve injury that were administered estradiol showed a lower paw withdrawal mechanical threshold and a shorter paw withdrawal thermal latency,indicating increased sensitivity to mechanical and thermal pain.Estrogen administration was also associated with increased expression of NMDAR1 immunoreactivity（as assessed by immunohistochemistry） and protein（as determined by western blot assay） in spinal dorsal root ganglia.This 17β-estradiol-induced increase in NMDAR1 expression was blocked by co-administration with AP-5,whereas AP-5 alone did not affect NMDAR1 expression.These results suggest that 17β-estradiol administration significantly reduced mechanical and thermal pain thresholds in rats with chronic constriction of the sciatic nerve,and that the mechanism for this increased sensitivity may be related to the upregulation of NMDAR1 expression in dorsal root ganglia.

2-氨基-1-甲基-1H-咪唑-5-羧酸乙酯的合成

以肌氨酸乙酯盐酸盐为起始原料,经氨酯交换反应、Claisen-Schmidt反应、合环反应共3步反应,得到目标产物2-氨基-1-甲基-1H-咪唑-5-羧酸乙酯(1),产物结构经^(1)H NMR确证。优化了反应条件:第一步,n_((肌氨酸乙酯盐酸盐))∶n_((K2)CO_(3))=1∶1.5,反应时间为8h,反应温度为25℃;第二步,n_((3))∶n_((NaH))=1∶1.2;第三步,n_((4))∶n_((NH2)CN)=1∶2.5,n_((4))∶n_((NaOAc))=1∶3.2,优化条件下的总收率为43.7%。此合成途径操作简便、产品质量好、总收率高,利于大量生产。