A novel detection of single-stranded DNA binding protein based on ss-DNA modified chip using surface plasmon resonance microscopy

An ss-DNA gold chip was prepared based on self-assembly of the thiol-derivatized oligonucleotide, and used for the determination of single-stranded binding protein （SSB） by surface plasmon resonance microscopy （SPR）. The experiment results showed that SSB binds ss-DNA with high specificity, and relative signal of SPR response is proportional to the concentration of SSB in the range of 0.1-100 ng/mL with a detection limit （S/N = 3） of 0.07 ng/mL.

Novel Halophyte EREBP/AP2-type DNA Binding Protein Improves Salt Tolerance in Transgenic Tobacco

EREBP/AP2-type proteins are members of a large DNA binding protein (DBP) family found in plants. Some members like APETALA2 and AtDREB/CBF can regulate flower development and response to environmental stresses, respectively. To characterize transcription factors involved in plant responses to salt stress, we constructed cDNA library from salt-treated halophyte (Atriplex hortensis) and isolated a novel gene encoding EREBP/AP2-type protein from this library. This cDNA contained an ORF of 723 bp and a long 3'-Untranslated-Region (UTR) of 655 bp. The deduced amino acid sequence showed one conserved DNA binding domain of EREBP/AP2, thus the corresponding gene was named AhDREB1 with a calculated molecular mass of 26.1 kD. AhDREB1 under the control of CaMV 35S promoter was then transformed into tobacco and nine independent transgenic lines were obtained and subjected to long term salt stress. The results suggested that overexpression of AhDREB1 improved the salt tolerance in transgenic tobacco through functioning as a regulatory molecule in response to salt stress. Analysis of Arabidopsis genome in database resulted in dozens of EREBP/AP2-type homologous proteins, of which seven members showed high similarity to AhDREB1. Secondary structure analysis predicted similar arrangement of a-helix in their DNA binding domains.

Endonuclease-rolling circle amplification-based method for sensitive analysis of DNA-binding protein

A sensitive approach for the qualitative detection of DNA-binding protein on the microarray was developed. DNA complexes in which a partial duplex region is formed from a biotin-primer and a circle single strand DNA （ssDNA） were spotted on a microarray. The endonuclease recognition site （ERS） and the DNA-binding sites （DBS） were arranged side by side within the duplex region. The working principle of the detection system is described as follows： when the DNA-binding protein capture the DBS, the endonuclease could not attach to the ERS, and the immobilized primer in the DNA complex could be extended along the circle ssDNA by rolling circle amplification （RCA）. When no protein protects the DBS, the ERS could be attacked by the endonuclease and subsequently no rolling circle amplification occurs. Thereby we can detect the sequence specific DNA-binding activity with high-sensitivity due to the signal amplification of RCA.

Chromodomain-helicase-DNA binding protein 5, 7 and pronecrotic mixed lineage kinase domain-like protein serve as potential prognostic biomarkers in patients with resected pancreatic adenocarcinomas

Pancreatic cancer is one of the deadliest cancers with a very poor prognosis. Recently, there has been a significant increase in research directed towards identifying potential biomarkers that can be used to diagnose and provide prognostic information for pancreatic cancer. These markers can be used clinically to optimize and personalize therapy for individual patients. In this review, we focused on 3 biomarkers involved in the DNA damage response pathway and the necroptosis pathway: Chromodomainhelicase-DNA binding protein 5, chromodomain-helicaseDNA binding protein 7, and mixed lineage kinase domain-like protein. The aim of this article is to review present literature provided for these biomarkers and current studies in which their effectiveness as prognostic biomarkers are analyzed in order to determine their future use as biomarkers in clinical medicine. Based on the data presented, these biomarkers warrant further investigation,and should be validated in future studies.

Endonuclease-based Method for Detecting the Sequence Specific DNA Binding Protein on Double-stranded DNA Microarray

The double-stranded DNA (dsDNA) probe contains two different protein binding sites. One is for DNA- binding proteins to be detected and the other is for a DNA restriction enzyme. The two sites were arranged together with no base interval. The working principle of the capturing dsDNA probe is described as follows: the capturing probe can be cut with the DNA restriction enzyme (such as EcoR I) to cause a sticky terminal, if the probe is not bound with a target protein, and the sticky terminal can be extended and labeled with Cy3-dUTP by DNA polymerase. When the probe is bound with a target protein, the probe is not capable to be cut by the restriction enzyme because of space obstruction. The amount of the target DNA binding proteins can be measured according to the variations of fluorescent signals of the corresponding probes.

REGULATED PHOSPHORYLATION OF THE GATA－2 DNA BINDINGPROTEIN IN ENDOTHELIAL CELLS

Endothelin-1 and a number of other genes expressd primarily in endothelial cells(EC)require a functional GATA element in their promoter region.The widely expressed zinc finger DNA binding protein GATA-2 has been characterized as the likely GATA factor which binds these GATA elements.To understand the specificity of this interaction,and to investigate the potential for regulation of GATA-2 activity,we have studied translation and post-translational modification of the GATA-2 protein. A specific antiserum immunoprecipitated a 52kDa GATA-2 protein from [35-S] methionine-labeled EC,as well as a wide variety of cultured human cell lines which express GATA-2 mRNA. Immunoprecipitation experiments with [32-P]-orthophosphate labeled cells indicated that GATA-2 is similarly phosphorylated in EC and non-EC lines. Thus the apparent cell-specific activity of this transcription factor is not regulated by translation or phosphorylation, and must derive from the interaction of GATA-2 with other nuclear proteins in the EC.Further studies investigated the potential regulation of GATA-2 phosphorylation in EC. Phosphoamino acid analysis indicated that GATA-2 is phosphorylated on serine and threonine residues in EC.The hasal phosphorylation of GATA-2 was rapidly and markedly increased when EC were treated with calcium ionophore A23187, while phorbol ester and forskolin had no effect.Phosphopeptide map analysis showed that A23187 induced phosphorylation of at least two additional sites in GATA-2.Gel shift assays employing nuclear extracts isolated from EC that had been treated with A23187 had a different DNA binding pattern when compared to control.This regulated phosphorylation of GATA-2 may provide a signaling pathway for hormonal regulation of endothelial cell genes such as endothelin-1 which alter their rate of transcription in response to increased intracellular calcium.

Identification and characterization of GIP1,an Arabidopsis thaliana protein that enhances the DNA binding affinity and reduces the oligomeric state of G-box binding factors

Environmental control of the alcohol dehydrogenase(Adh)and other stress response genes in plants is in part brought about by transcriptional regulation involving the G-box cis-acting DNA element and bZIP G-box Binding Factors(GBFs).The mechanisms of GBF regulation and requirements for additional factors in this control process are not well understood.In an effort to identify potential GBF binding and control partners,maize GBF1 was used as bait in a yeast two-hybrid screen of an A.thaliana cDNA library.GBF Interacting Protein 1(GIP1)arose from the screen as a 496 amino acid protein with a predicted molecular weight of 53,748 kDa that strongly interacts with GBFs.Northern analysis of A.thaliana tissue suggests a 1.8-1.9 kb GIP1 transcript,predominantly in roots.Immunolocalization studies indicate that GIP1 protein is mainly localized to the nucleus.In vitro electrophoretic mobility shift assays using an Adh G-box DNA probe and recombinant A.thaliana GBF3 or maize GBF1,showed that the presence of GIP1 resulted in a tenfold increase in GBF DNA binding activity without altering the migration,suggesting a transient association between GIP1 and GBF.Addition of GIP1 to intentionally aggregated GBF converted GBF to lower molecular weight macromolecular complexes and GIP1 also refolded denatured rhodanese in the absence of ATP.These data suggest GIP1 functions to enhance GBF DNA binding activity by acting as a potent nuclear chaperone or crowbar,and potentially regulates the multimeric state of GBFs,thereby contributing to bZIP-mediated gene regulation.

Role of the PEST sequence in the long-type GATA-6 DNA-binding protein expressed in human cancer cell lines

GATA-6 mRNA utilizes two Met-codons in frame as translational initiation codons in cultured mammalian cells. Deletion of the nucleotide sequence encoding the PEST sequence between the two initiation codons unusually reduced the protein molecular size on SDS-polyacrylamide gel-electrophoresis. The reduced molecular size is ascribed to the molecular property of GATA-6, since both amino-and carboxy-lterminal tags introduced into GATA-6 were detected on the gel. This PEST sequence seems to contribute to expansion of the long-type GATA-6 molecule. The long-type GATA-6 containing the PEST sequence exhibits more activation potential than that without this sequence, the latter’s activity being similar to that of the short-type GATA-6. We further demonstrated that human colon and lung cancer cell lines express both the long-type GATA-6 and the short-type GATA-6 in their nuclei.

Isolation and identification of proteins binding to the major breakpoint region(mbr) of bcl2 gene

Objective： We have previously found that mbr is a regulatory element of the bcl2 gene. The objective of this study is to isolate and identify the proteins binding to the 37 mbr in the 3 ＇ -end of the mbr. Methods： Streptavidin magnetic particles were ligated to concatameric oligonucleotides of 37 mbr and incubated with the nuclear extracts of Jurkat cells. The DNA-binding proteins were eluted and then resolved by SDS-PAGE. After silver staining, the protein bands were excised and subjected to MALDI-TOF MS. Results： Several protein bands were detected after the isolation with magnetic particles, and Splicing factor, proline- and glutamine-rich（SFPQ）, Poly（ADP-ribose） polymerase I（PARP）, and promyelocytic leukemia protein（PML） were identified by MALDI-TOF MS. Conclusion： Several proteins were isolated and identified from the 37 mbr-protein complex. Results of this study establish a foundation for further study of the mechanisms by which mbr executes its regulatory function.

Presence/Absence of Two Types of Z-DNA Binding Domains in the Genomes of Organisms from Archaea, Bacteria, and Eukaryotes and Its Implications

We conducted genome sequence analysis to examine the presence/absence of two types of Z-DNA binding domains in various organisms. We examined 68 organisms from archaea, 914 organisms from bacteria, and 199 organisms from eukaryotes. RecA protein from Escherichia coli has a Z-DNA binding domain and this protein promotes homologous recombination. All the organisms examined had this domain. This result indicated that this domain is essential for all the organisms. RNA editing enzyme, adenosine deaminase from human has another type of Z-DNA binding domain. This domain was observed in some organisms of archaea, bacteria, and eukaryotes. The presence/absence of Z-DNA binding domain in adenosine deaminase indicated that gain and loss of this domain had occurred in the process of evolution. The implication of presence and absence of this domain is discussed in this study.

Taq DNA聚合酶的分子改造及其在探针法qPCR直扩体系中的应用

Taq DNA聚合酶作为实时荧光定量聚合酶链式反应(qPCR)技术的核心组分,其性能优劣直接影响qPCR技术的进一步发展。然而,野生型Taq DNA聚合酶的耐抑制剂性能差、延伸性能不足。为获得具有高性能的Taq DNA聚合酶,采用基因工程技术将双链DNA结合蛋白Sso7d或Sto7d融合在野生型Taq DNA聚合酶的N端或C端,构建了4个均可溶表达的改造体,再经过耐受性测试筛选较优的改造体,结果显示:改造体Taq-Sto的耐受性最高,其热稳定性不受影响,且在1 s/kbp的延伸条件下能成功扩增靶标,表明Taq-Sto具有增强的延伸性能,在TaqMan探针法qPCR体系中对腐殖酸、单宁酸、全血等抑制剂同样表现出良好的耐受性。EMSA实验发现:Taq-Sto对DNA模板的结合亲和力有所提高,有利于增强Taq-Sto对模板的竞争力;将Taq-Sto应用于非洲猪瘟病毒(ASFV)的TaqMan探针法qPCR检测,与商品化试剂相比,Taq-Sto具有更低的ASFV检出限,且在体积分数为2%~6%的猪粪便样本或猪肉样本中的检测灵敏度分别为100.0%和85.4%,说明Taq-Sto在直扩qPCR检测领域更具有优势。

精神分裂症患者血清反式激活反应-DNA结合蛋白表达水平与临床症状的相关性研究

目的:探讨精神分裂症患者血清反式激活反应-DNA结合蛋白(trans activated response DNA binding protein,TDP43)表达水平与临床症状的相关性研究。方法:选取2020年10月至2021年10月于本院确诊收治的54例精神分裂症患者为研究对象,记为研究组,同时以80名健康体检者作为对照组。收集研究组、对照组的一般临床资料和阳性与阴性症状量表(positive and negative syndrome scale,PANSS)评分进行比较,采集两组静脉血,分析血清TDP43水平和生化指标;Pearson法和Logistic回归分析一般病理症状评分、阴性症状量表评分、阳性症状量表评分及PANSS总分与血清TDP43水平的相关性及精神分裂症患者发生的危险及保护因素。结果:研究组、对照组在高密度脂蛋白、性别、受教育时间、年龄、总胆固醇、体质量指数、吸烟、三酰甘油及血糖方面比较,差异均无统计学意义(P均>0.05);与对照组相比,研究组人员低密度脂蛋白显著降低,患者血清TDP43水平以及一般病理症状评分、阴性症状量表、阳性症状量表评分及PANSS总分、同型半胱氨酸均显著增加(P均<0.05)。相关性分析显示,血清TDP43水平与一般病理症状评分、阴性症状量表评分、阳性症状量表评分及PANSS评分均呈正相关性(P均<0.05)。多因素Logistic分析显示,血清TDP43水平、PANSS评分、低密度脂蛋白、同型半胱氨酸为精神分裂症患者发生的影响因素(P均<0.05)。结论:精神分裂症患者血清TDP43水平显著升高,与临床症状有关。

Bacterial ArtA protein specifically binds to the internal region of IS1 <i>in vitro</i>

The internal region of bacterial translocatable IS1 acts as a cis-element to stimulate transcription from the various promoters located upstream. The product of the artA gene is genetically shown to stimulate transcription with the cis-element. Here, a codon-optimized artA gene was synthesized and cloned to express the ArtA protein. ArtA was purified as the Histagged protein. Nitrocellulose filter binding assay showed that ArtA specifically binds to the IS1 internal region. Electrophoretic mobility shift assay also showed specific binding of ArtA to the IS1 internal region. These results imply that ArtA directly binds to the IS1 internal region and stimulates transcription.

Affinity chromatography-dependent selection (ACDS)of genomic DNA fragments bound specifically to bacterial synthesized Myc/Myn proteins

This paper describes an approach to seek for mouse c-Myc/Myn proteins-bound specific sequences among ge-nomic DNA. cDNA fragment of myn gene was obtained through RT-PCR technique from RNA of NIH3T3 cells. DNA fragments encoding BR/HLH/LZ structure of Myc and Myn proteins were cloned in frame into pGEX-2T vec-tor respectively Fusion GST-Myc and GST-Myn synthe-sized in E.coli hosts showed affinity to CACGTG E-boxDNA and subsequently interacted with genomic fragments prepared through whole-genome-PCR. A PCR-assisted procedure which combines protein-DNA interaction and affinity chromatography was designed to enrich Myc/Myn bound DNA. At least two genomic DNA fragments ob- tained exhibit specifical binding capacity to Myc/Myn complex but not to GST alone. Significance of the work and of the technique itself as well as identification of the DNAs are discussed.

Determination of Interaction between NFκB p50 and <i>β</i>-IFN-<i>κ</i>B Binding Oligo Using AlphaLISA in HTP Fashion

NF-κB plays a crucial role in regulating various biological processes including innate and adaptive immunity, inflammation, stress responses, B-cell development, and lymphoid organogenesis. Currently, several assays like electrophoretic mobility shift assay (EMSA), enzyme-linked immunosorbent assay (ELISA), fluorescence resonance energy transfer (FRET) and time-resolved fluorescence resonance energy transfer (TR-FRET) are widely used for studying the NFκB intraction with β-IFN-κB binding oligo. Each of these techniques has varying utility with distinct strengths and weaknesses. We describe a method AlphaLISA to identify NFκB p50 protein and β-IFN-κB binding oligo sequence and interaction is efficient at a given concentration (10 nM) in the EMSA and Biacore’s SPR assays. The method has many advantages such as use of small volume, high throughput (HTP), convenience of sample preparation and data analysis.

急性脑出血患者血清E盒锌指结合蛋白1及DNA甲基化转移酶1与神经功能缺损和预后的相关性分析

目的探讨急性脑出血(ACH)患者血清E盒锌指结合蛋白1(ZEB1)、DNA甲基化转移酶1(DNMTl)与神经功能缺损、预后的关系。方法选取2019年7月—2022年7月本院收治的105例ACH患者为ACH组,依据ACH患者入院时美国国立卫生研究院卒中量表(NIHSS)评分将其分为轻度组(n=34)、中度组(n=41)、重度组(n=30)。根据改良Rankin量表(mRS)评分将ACH患者分为预后良好组(n=65)和预后不良组(n=40)。另纳入同期105例体检健康者为对照组。选取2021年7月—2022年7月本院诊治的45例ACH患者对构建的ACH预后模型的受试者工作特征(ROC)曲线进行验证。采用酶联免疫吸附试验检测血清ZEB1、DNMT1水平;采用Spearman法分析ACH患者ZEB1、DNMT1水平与NIHSS评分的关系;采用多因素Logistic回归模型分析ACH患者预后的影响因素,采用ROC曲线评估血清ZEB1、DNMT1水平对ACH患者预后的预测价值。结果与对照组相比,ACH组血清ZEB1、DNMT1水平升高,差异有统计学意义(P<0.05)。与轻度组相比,中度组和重度组ACH患者血清ZEB1、DNMT1、NIHSS评分均升高,差异有统计学意义(P<0.05);与中度组相比,重度组ACH患者血清ZEB1、DNMT1、NIHSS评分均升高,差异有统计学意义(P<0.05)。Spearman分析结果显示,ACH患者血清ZEB1、DNMT1水平与NIHSS评分均呈正相关(r=0.569、0.763,P均<0.001)。单因素分析结果显示,与预后良好组比较,预后不良组患者NIHSS评分、血肿体积、ZEB1及DNMT1水平均升高或增大,差异有统计学意义(P<0.05)。Logistic回归分析结果显示,ZEB1、DNMT1、NIHSS评分、血肿体积增大是ACH患者预后不良的危险因素(P<0.05)。血清ZEB1、DNMT1预测ACH患者预后的曲线下面积(AUC)分别为0.834、0.854,ZEB1、DNMT1联合预测ACH患者预后的AUC为0.944,灵敏度为95.0%,特异度为86.2%。以验证组人群对预测预后的ROC曲线进行验证,结果显示AUC为0.903(95%CI:0.854~0.951),提示预后预测曲线具有较好的区分度。结论ACH患者血清ZEB1、DNMT1水平较高,二者均与ACH患者神经功能缺损、预后显著相关,且血清ZEB1、DNMT1联合可能更有利于临床评估ACH患者预后情况。

补阳还五汤提高血管性痴呆大鼠海马CREB、C/EBP的DNA结合活性

目的观察补阳还五汤对血管性痴呆大鼠海马CREB(cAMP反应元件结合蛋白)、C/EBP(CCAAT/增强子结合蛋白)DNA结合活性的影响。方法实验分为假手术组、模型组、补阳还五汤组和尼莫地平组。采用改良的4血管法制备血管性痴呆模型,分别给予生理盐水、补阳还五汤、尼莫地平灌胃干预,用凝胶电泳迁移率改变分析法(EMSA)测定各组大鼠CREB和C/EBP的DNA结合活性。结果与假手术组比较,模型组大鼠海马组织CREB的DNA结合活性明显降低(P<0.01);与模型组比较,尼莫地平组与补阳还五汤组明显升高(P<0.01);尼莫地平组与补阳还五汤组之间差异无显著性(P>0.05)。结论补阳还五汤可提高VD大鼠海马组织CREB、C/EBP与DNA的结合活性。

日本血吸虫DNA多价疫苗pVIVO_2SjFABP-23的构建及其保护性免疫

目的构建日本血吸虫多价DNA疫苗pVIVO2SjFABP-23,并观察其在小鼠抗血吸虫感染中的免疫保护作用。方法根据Sj FABP和Sj23的基因序列合成两对特异性引物,利用重组PCR技术将日本血吸虫Sj FABP和Sj23的基因片段进行拼接,得到融合基因SjFABP-23,再将该片段重组于p GEM-T载体中,进行PCR扩增及DNA序列测定。然后经双酶切将目的片段SjFABP-23克隆到pVIVO2的一个多克隆位点上转化E.coliGT 110获得重组质粒pVIVO2SjFABP-23,免疫小鼠进行免疫保护性实验。结果PCR扩增出一条大小约为1.1Kb的目的片段。免疫小鼠获得52.14%减虫率(P<0.01)和60.93%的减卵率(P<0.01),且均高于单价疫苗pVIVO2Sj23(P<0.05)。结论PCR成功扩增SjFABP-23的基因片段,血吸虫DNA多价疫苗pVI-VO2SjFABP-23构建成功,该疫苗在小鼠抗血吸虫感染中具有比单价疫苗pVIVO2Sj23更好的免疫保护作用。

日本血吸虫脂肪酸结合蛋白DNA疫苗诱导小鼠保护性免疫力的研究

目的构建日本血吸虫脂肪酸结合蛋白(Sj14FABP)重组质粒,并观察其在小鼠体内诱导的抗日本血吸虫感染保护作用。方法RT-PCR特异性扩增Sj14FABP基因,将其克隆入真核表达载体pVIVO2,通过PCR、双酶切及测序鉴定。获得的重组质粒pVIVO2-Sj14FABP转染HepG2细胞,间接免疫荧光(IFA)检测蛋白表达;并免疫BALB/c小鼠,30d后攻击感染,感染后45天剖杀,计数检获成虫数和肝脏虫卵数。结果RT-PCR扩增出大小为440bp的Sj14FABP片段,重组质粒经PCR和双酶切后均获得目的片段,转染细胞IFA结果显示有较强荧光。重组质粒免疫小鼠后分别获得24.1%减虫率和27.2%减卵率。结论成功构建和表达重组质粒pVIVO2-Sj14FABP,该核酸疫苗能够诱导小鼠产生部分抗血吸虫感染的保护力。

日本血吸虫DNA多价疫苗SjGST-FABP/pcDNA3的构建及其保护性免疫研究

目的构建日本血吸虫DNA多价疫苗SjGST-FABP/pcDNA3,用以免疫小鼠,观察其在小鼠抗血吸虫感染中的免疫保护作用。方法根据质粒pGEX-4T-1中SjGST-ORF和SjFABP基因序列,利用基因重组、PCR等技术将SjGST和SjFABP编码基因拼接在一起,得到融合基因SjGST-FABP,将融合基因SjGST-FABP定向克隆到pcDNA3多克隆位点上,转化大肠杆菌,经质粒扩增和DNA序列测定后,进行小鼠动物免疫和日本血吸虫尾蚴攻击感染及免疫保护性评价。结果成功构建了日本血吸虫DNA多价疫苗SjGST-FABP/pcDNA3。免疫小鼠获得42.39%的减虫率和56.09%肝减卵率(P<0.05)。结论日本血吸虫DNA多价疫苗SjGST-FABP/pcDNA3可诱导部分抗血吸虫尾蚴攻击感染的免疫保护效果,具有疫苗研究与开发价值。