A Preliminary Study on Genetic Variation of g E Gene of an Epidemic Pseudorabies Virus Strain and Its Pathogenicity to Piglets

[Objective] This study aimed to investigate the genetic variation of g E gene of an epidemic pseudorabies virus（PRV） strain and its pathogenicity to piglets. [Method] By serial passage in Vero cells, a PRV strain was isolated from the brain tissues of stillborn fetuses delivered by sows with suspected PRV infection and preliminarily identified by PCR. g E gene of the isolated PRV strain was amplified and sequenced for phylogenetic analysis. In addition, the pathogenicity of the isolated PRV strain to 6-week-old piglets was evaluated. [Result] A PRV strain was successfully isolated and named PRV N5 B strain, which could proliferate in Vero cells and TCID50 of the 15 thgeneration virus liquid reached 10^7.125/0.1 ml. Specific bands could be amplified by PCR. g E gene in the isolated PRV strain was 1 740 bp in length. A phylogenetic tree was constructed based on full-length g E sequences, which showed that PRV N5 B strain and PRV strains isolated since 2012 were clustered into the same independent category and shared 99.7%-100% homology of nucleotide sequences. Compared with related sequences published previously, there were insertions of three consecutive bases at two loci. Animal experiments showed that intranasal inoculation of 6-week-old piglets with 2 ml of PRV N5 B strain（10^6/0.1 ml） led to a mortality rate of 100%. [Conclusion] In this study,genetic variability of g E gene in PRV N5 B isolate and its pathogenicity to piglets were analyzed, which provided a theoretical basis for the development of new vaccines to prevent and control porcine pseudorabies.

Construction of Recombinant Pseudorabies Virus Expressing Canine Distemper Virus H Gene and Analysis on Its Biological Characters

[Objective] The aim was to construct a recombinant pseudorabies virus expressing canine distemper virus H gene and investigate its biological characters.[Method] H gene of canine distemper virus（CDV）strain Onderstepoort was produced by RT-PCR,inserted into pcDNA3.1（＋）vector to construct a expression cassette,which was then subcloned into transfer vector p8AA,prior to the insertion of LacZ expression cassette.The resulting new transfer vector was named as p8AAZH.Subsequently,p8AAZH was co-transfected with the genome of pseudorabies virus（PRV）Bartha-K61 into BHK-21 cells to enable gene recombination and virus package,and the virus solution was collected as cytopathic effect occurring.A series of procedures including blue plaque purification,PCR identification,observation under electron microscope and Western blot were carried out to screen the recombinant pseudorabies virus and identify the protein expression of target gene.Meanwhile,growth curve of the recombinant virus was determined in BHK-21 cells.[Result] The H gene had been inserted into the genome of Bartha-K61 strain,and RPRV-H was the same as Bartha-K61 in the one-step growth curve and cytopathic effect in BHK-21 cells.[Conclusion] The recombinant pseudorabies virus was constructed,and the insertion of H gene did not influence proliferation of recombinant virus,which laid a foundation for development of recombinant canine distemper virus vaccine.

Expression of Pseudorabies Virus gE Core Epitopes in Escherichia coli Strain BL21 and Utilization of Indirect PRV gE-ELISA

Pseudorabies virus glycoprotein E （PRV gE） has been recognized as a suitable diagnostic antigen for pseudorabies. In order to produce gE antigen in large quantities and at low cost, a gene fragment encoding PRV gE core epitopes was expressed in E. coli BL21 expression system. SDS-PAGE and Western Blotting revealed that the expression product in culture supematant of E. coli BL21 was a recombinant protein, approximately 51.8 Kd. At 5 h post-induction, protein concentration assay showed that the expression product amounted to 1.65 mg/ml, accounting for 24. 17% of total proteins in the culture supematant. An indirect PRV gE-ELISA was established by using the recombinant expression product as a coating antigen. Cross-reactivity assay showed that this antigen was PRV specific. In addition, the assay was consistently reproducible. Comparison of detection results of 240 serum samples between PRV gE-ELISA and a commercially available PRV diagnostic kit showed that there was no significant difference between these two methods （P 〉 0.05 ）.

Subculturing cells have no effect on CRISPR/Cas9-mediated cleavage of UL30 gene in pseudorabies virus

CRISPR/Cas9-mediated genome editing can inhibit virus infection by targeting the conserved regions of the viral genomic DNA. Unexpectedly, we found previously that pseudorabies virus(PRV) could escape from CRISPR/Cas9-mediated inhibition.In order to elucidate whether the escape of PRV from Cas9-mediated inhibition was due to cell deficiencies, such as genetic instability of sgRNA or Cas9 protein, the positive cells were passaged ten times, and PRV infection in the sgRNA-expressing cells was evaluated in the present study. The results showed that subculturing cells has no effect on Cas9-mediated cleavage of PRV. Different passages of PX459-PRV cells can stably express sgRNA to facilitate Cas9/sgRNA cleavage on the UL30 gene of PRV, resulting in a pronounced inhibition of PRV infection. Studies to elucidate the mechanism of PRV escape are currently in progress.

Development of PPA-ELISA for Detecting Antibodies against Porcine Pseudorabies Virus Using Truncated Recombinant Glycoprotein gD Expressed in E.coli

The purpose of this study was to develop a method for detecting antibodies against porcine pseudorabies virus （PRV）. According to the published genomic sequence of PRV SA strain, an approximately 1 070-bp gD gene fragment was amplified by PCR. The PCR products were cloned into the prokaryotic expression vector pET30a and the positive recombinant plasmid was transformed into E. coli BL21. Through induction with IPTG, the recombinant gD protein was expressed as inclusion bodies. As analyzed by western blot assay, the purified recombinant gD protein had good antigenicity and high specificity. Using the purified gD protein as coating antigen and horseradish peroxidase labeled staphylococcal protein A （PPA） as secondary antibody, we developed a PPA-ELISA for detecting antibodies against porcine PPV. No cross-reaction with the positive sera against seven common pathogens in pigs including classical swine fever virus, porcine parvovirus, porcine reproductive and respiratory syndrome, Japanese encephalitis virus, porcine circovirus type 2, porcine epidemic diarrhea virus, transmissible gastroenteritis virus was observed. The repeatability test showed that the intra- and inter-assay coefficients of variation were lower than 5% and 10%, respectively. Compared with the ELISA gD antibody test kit produced by IDEXX, the coincidence, sensitivity and specificity of the developed PPA-ELISA were 92.0%, 95.1% and 88.1%, respectively. The developed PPA-ELISA had good repeatability, sensitivity and specificity and was a rapid and simple serological method for surveillance of PRV antibodies in pig herds as well as for rapid diagnosis and epidemiological investigation of PRV infection.

SphK1/S1P/S1PR2信号通路促进肌生成:运动改善骨骼肌健康的新视角

背景:近年来,运动改善骨骼肌的健康已成为学者们关注的一个重要研究内容,适宜的运动对骨骼肌具有积极的作用,其中在运动激活鞘氨醇激酶1(sphingosine kinase1,SphK1)/鞘氨醇-1-磷酸(sphingosine-1-phosphate,S1P)/鞘氨醇-1-磷酸受体2(sphingosine-1-phosphate receptor2,S1PR2)信号通路如何改善骨骼肌的健康,正受到科研人员的重视。目的:研究运动经SphK1/S1P/S1PR2信号通路如何改善骨骼肌的健康,探索治疗相关肌肉疾病的新方法,以改善人的骨骼肌健康。方法:检索Web of Science、PubMed、中国知网、万方和维普数据库从建库至今与文章主题相关的文献,以“signaling pathway,SphK1,S1P,S1PR2,skeletal muscle,satellite cell,myogenesis,exercise”为英文检索词,以“信号通路,SphK1,S1P,S1PR2,骨骼肌,卫星细胞,肌生成,运动”为中文检索词,最终纳入69篇文献进行分析。结果与结论:①SphK1/S1P/S1PR2信号通路是一个复杂的调控网络,通过SphK1催化产生的S1P,与S1PR2等受体的相互作用,触发下游信号转导过程,进而调控细胞、组织、器官和系统的多种生物学功能。②SphK1/S1P/S1PR2信号通路能调控卫星细胞增殖和成肌细胞分化,改善肌生成。③文章通过文献资料调研法分析了SphK1/S1P/S1PR2信号通路的生理基础以及运动对其影响的可能性。急性有氧运动可提高骨骼肌中SphK1的表达,人体和动物研究中已证实急性和长期运动均可提高骨骼肌中S1P水平,另外研究表明长期抗阻运动可提高S1PR2在骨骼肌中的表达,部分实验结果表明急性和长期运动对肌肉或者血液中S1P水平无显著影响,出现不同结果的原因可能是选择的研究对象、方式、强度及频率不同,而具体机制尚不明确。④研究认为,运动能够促进SphK1/S1P/S1PR2信号通路在骨骼肌中的表达,调控下游相关信号通路,并且针对这一信号通路的研究可能为骨骼肌疾病的治疗提供新的策略和方法,从而改善骨骼肌健康。⑤未来应深化对SphK1/S1P/S1PR2信号通路与骨骼肌健康关联的研究,进一步揭示其与卫星细胞、成肌细胞的调控关系及与上下游通路的相互作用,挖掘其临床应用价值,制定康复方案时考虑该通路变化,探索不同运动对该通路的影响机制,并将其作为潜在治疗靶点,结合人体肌肉模型提升研究深度和准确性。

2型糖尿病患者心电图PR、QT、QTc间期延长与颈动脉粥样硬化相关性研究

目的:探讨心电图PR、QT、QTc间期延长与2型糖尿病(T2DM)患者发生颈动脉粥样硬化的关系。方法:采用病例对照研究方法,选取97例确诊为T2DM且伴有颈动脉粥样硬化(CAS)的患者作为CAS组,选取确诊为T2DM但颈动脉未发现粥样硬化的95例患者作为对照组,比较两组患者的心电图PR、QT、QTc间期测定值、血糖血脂等,采用多因素分析方法探讨心电图PR、QT、QTc间期延长与T2DM患者发生颈动脉粥样硬化形成的关系。结果:CAS组患者的PR、QT、QTc时间均长于对照组患者,差异具有统计学意义(均P<0.05);CAS组患者的糖尿病病程长于对照组患者,CAS组患者中合并冠心病的占比高于对照组,差异具有统计学意义(均P<0.05);CAS组患者的血清甘油三酯(TG)、总胆固醇(TC)、高敏感度C-反应蛋白(hs-CRP)、丙氨酸氨基转移酶(ALT)水平均高于对照组患者,差异具有统计学意义(均P<0.05)。PR延长(OR=1.833)、QT延长(OR=1.718)、QTc延长(OR=1.487)、TG增高(OR=1.833)、hs-CRP增高(OR=2.081)、糖尿病病程延长(OR=2.036)是T2DM患者发生颈动脉粥样硬化的独立危险因素(均P<0.05)。结论:T2DM患者心电图PR、QT、QTc间期延长与发生颈动脉粥样硬化密切相关,可以作为早期监测患者颈动脉粥样硬化病变的筛选指标。

Research Progress on Pseudorabies Gene-deleted Vaccine

Pseudorabies is caused by pseudorabies virus (PrV), which is a member of family Herpesviridae, subfamily Alphaherpesvirinae and is the agent of acute infectious disease in many domestic and wild animals. Swine was the natural host and reservior of PRV, which inflicts major economic loss in pig industries world wide. Immunization with safe, effective vaccine is main measurements to prevent the disease. In this assay, research progress on PRV gene-deleted vaccine used extensively today was discussed.

Detection of Serum Antibodies of Porcine Pseudorabies Virus(PRV)in Binzhou City in 2014

To understand immunization effect of pseudorabies vaccine and infection status of porcine pseudorabies （PR） in pig farms and guide prevention and control against PR, 453 copies of blood samples collected from 43 different scale pig farms in four counties （districts） of Binzhou City were detected with ELISA to investigate PRV gB antibody and gE antibody. Detection results showed that the gB antibody positive rate of sows was 75.58%, and that of fattening pigs was 68.67% ; the pig farms with positive rate higher than 70% accounted for 74.42% of total survey pig farms. The PRV gE antibody positive rates of sows and fatte- ning pigs were 25.41% and 26.67%, and the positive rates of pig farms were 46.51% and 44.33%, respectively. There were regional differences among counties （districts）.

Development of Multi-PCR for Differentiation of Vaccine Strain and Field Isolate of Porcine Pseudorabies Virus

Three pairs of primer were designed for amplification of porcine pseudorabies virus （PRV） gB, gE, and TK gene by multiplex PCR （multi-PCR） in order to differentiate vaccine strains from field isolates. Three specific bands were obtained respectively at the expected size, 427 bp （gB gene）, 298 bp （gEgene）, and 208 bp （TKgene）, Then four different gene-deleted vaccines of PRV were detected by multi-PCR. One ex- pected specific band was observed in one of samples, while two bands in the others. As shown by the detection results, the multi-PCR has high sensitivity and specificity and should be applied in pathogen diagnosis and epidemiological investigation in the future.

Pr,Yb,Ho:GdScO_(3)晶体生长及光谱性能

2.7-3.0μm波段激光在很多领域具有重要应用,为探索和发展该波段新型晶体材料,本文采用提拉法生长出Pr,Yb,Ho:GdScO_(3)晶体,通过共掺入Pr3+离子以达到衰减Ho^(3+):^(5)I_(7)能级寿命的目的.采用X射线衍射测试得到了晶体的粉末衍射数据,测量了拉曼光谱,并对晶体的拉曼振动峰进行指认,对Pr,Yb,Ho:GdScO_(3)晶体的透过光谱、发射光谱和荧光寿命进行表征.Yb^(3+)的最强吸收峰在966 nm,吸收峰半峰宽为90 nm;2.7-3.0μm波段最强发射峰在2850 nm,半峰宽为70 nm;Ho^(3+):^(5)I_(6)和^(5)I_(7)能级寿命分别为1094μs和56μs.与Yb,Ho:GdScO_(3)晶体相比,Yb^(3+)的吸收峰和2.7-3.0μm的发射峰半峰宽明显展宽,同时下能级寿命显著减小,计算表明Ho^(3+):^(5)I_(7)与Pr^(3+):^(3)F_(2)+^(3)H_(6)能级之间能实现高效的能量传递.以上结果表明Pr,Yb,Ho:GdScO_(3)晶体是性能更优异的2.7-3.0μm波段激光材料.

T6态ZL105-(Pr+Ce)合金的组织及力学性能研究

采用光学显微镜、扫描电子显微镜、EDS分析仪、布氏硬度与拉伸试验研究了混合稀土与T6热处理对ZL105合金的微观组织及力学性能的影响。结果表明,当添加0.5wt%的稀土(Pr+Ce)后,ZL105合金的α-Al相、共晶Si相及富Fe相均被细化。ZL105-0.5wt%(Pr+Ce)合金经T6热处理后,α-Al相进一步细化,晶粒趋于圆整,共晶Si相也进一步细化,由长条状转变为短颗粒状,但是富Fe相的形貌和尺寸没有发生明显变化。T6态ZL105-0.5wt%(Pr+Ce)合金的抗拉强度、伸长率及硬度分别为257.7 MPa、7.0%、98 HB。T6态ZL105-0.5wt%(Pr+Ce)合金的断口为典型的塑性断裂特征,断口表面出现了许多韧窝,主要以小韧窝为主,分布较均匀且密集。T6热处理后合金的力学性能得到了显著改善。

miR-592靶向调控PRDM5影响肾细胞癌侵袭转移及自噬的机制研究

目的探究miR-592靶向调控PR结构域锌指蛋白5(PR domain zinc finger protein 5,PRDM5)影响肾细胞癌(renal cell carcinoma,RCC)侵袭转移及自噬的机制。方法RT-qPCR、蛋白质印迹检测RCC组织和细胞中miR-592、PRDM5 mRNA和蛋白水平。A498、786-O细胞分为anti-miR-NC组、anti-miR-592组、anti-miR-592+si-NC组、anti-miR-592+si-PRDM5组。RNA免疫共沉淀(RIP)检测miR-592和PRDM5的结合;CCK-8、Transwell实验检测细胞增殖、迁移和侵袭能力;透射电镜观察自噬小体形成;蛋白质印迹检测细胞PRDM5、基质金属蛋白酶(MMP)-2、MMP-9、Beclin1、微管相关蛋白1轻链3(LC3)Ⅱ/Ⅰ水平。建立移植瘤裸鼠模型,分析敲低miR-592表达对移植瘤生长的影响。结果RCC组织和细胞中PRDM5 mRNA和蛋白水平降低,miR-592水平增加(P<0.05)。敲低miR-592表达后,细胞A_(450 nm)、迁移和侵袭细胞数、MMP-2、MMP-9水平降低,自噬小体数量、Beclin1、LC3Ⅱ/Ⅰ水平增加(P<0.05)。敲低PRDM5表达能部分逆转敲低miR-592对细胞增殖、侵袭及自噬的影响(P<0.05)。敲低miR-592表达能够抑制裸鼠移植瘤生长(P<0.05)。结论miR-592通过靶向抑制PRDM5表达,促进RCC细胞增殖、侵袭转移能力,并抑制自噬能力。

3PR参与式健康教育在老年急性上消化道出血患者治疗中的应用价值

目的探究以参与式研究(participatory research,PR)为基础模块、参与式角色扮演(participatory role-playing,PR)为核心模块、参与式总结(participatory review,PR)为强化模块(简称3PR)的参与式健康教育在老年急性上消化道出血(acute upper gastrointestinal bleeding,AUGIB)患者的应用价值。方法选择2020年1月-2023年6月南京市第二医院急诊科收治的老年AUGIB患者80例,按随机数字表法分成观察组(n=40)和对照组(n=40)。在病情稳定后,对照组采用常规健康教育,观察组采用3PR参与式健康教育。比较2组疾病认知、自我感知负担量表(SPBS)评分、Morisky用药依从性量表(MMAS-8)评分、遵医行为、生活质量综合评定问卷(GQOLI-74)评分和再出血率差异。结果干预后,2组疾病认知、遵医行为、GQOLI-74量表各维度评分均高于同组干预前,SPBS量表各维度评分均低于同组干预前,且观察组改善程度大于对照组,差异均有统计学意义(P<0.05);观察组用药依从率高于对照组(P<0.05);随访3个月,观察组再出血率低于对照组(P<0.05)。结论3PR参与式健康教育对老年AUGIB患者的干预效果显著,可有效提高疾病认知水平和用药依从性,减轻患者自我感知负担,改善遵医行为,提高生存质量,减少疾病复发。

基于PR—Henry改进模型的酸性天然气——地层水体系及其相平衡特征分析

准确表征酸性天然气—地层水体系的相平衡规律,对于天然气开发过程中的水溶气量和凝析水量分析具有重要意义,但目前常用的PR状态方程与Henry定律等理论对酸性天然气—地层水体系的相平衡研究还存在不适用的问题。为进一步考虑酸性气体和地层水矿化度对体系相平衡的影响,改进并提高对天然气溶解度和饱和含水量的计算精度,在PR状态方程与Henry定律相结合建立的PR—Henry模型基础上,考虑了溶解盐对体系相平衡的影响,采用定标粒子理论(SPT)修正了Henry常数,建立了改进的PR—Henry模型,最后分析了天然气组成、压力、温度和盐水含盐量对天然气溶解量和饱和含水量的影响。研究结果表明:(1)模型计算结果与实测资料对比,平均相对偏差分别为5.3%和4.55%,表明该模型能够应用于不同温度、压力和组成的酸性天然气-地层水体系的相平衡计算;(2)天然气在地层水中的溶解量受天然气组成、温度、压力和地层水含盐量的影响;(3)天然气饱和含水量受温度和压力影响十分明显。结论认为,改进的PR—Henry模型为天然气开采过程评价和CO_(2)埋存溶解量计算提供了一种有效的方法,对于评估天然气可采储量及开发特征具有重要的参考意义。

Pathogenicity of a currently circulating Chinese variant pseudorabies virus in pigs

AIM:To test the pathogenicity of pseudorabies virus(PRV)variant HN1201 and compare its pathogenicity with a classical PRV Fa strain.METHODS:The pathogenicity of the newly-emerging PRV variant HN1201 was evaluated by different inoculating routes,virus loads,and ages of pigs.The classical PRV Fa strain was then used to compare with HN1201 to determine pathogenicity.Clinical symptoms after virus infection were recorded daily and average daily body weight was used to measure the growth performance of pigs.At necropsy,gross pathology and histopathology were used to evaluate the severity of tissue damage caused by virus infection.RESULTS:The results showed that the efficient infection method of RPV HN1201 was via intranasal inoculation at 107 TCID50,and that the virus has high pathogenicity to 35-to 127-d old pigs.Compared with Fa strain,pigs infected with HN1201 showed more severe clinical symptoms and pathological lesions.Immunochemistry results revealed HN1201 had more abundant antigen distribution in extensive organs.CONCLUSION:All of the above results suggest that PRV variant HN1201 was more pathogenic to pigs than the classical Fa strain.

麦冬皂苷D调节SphK1/S1P/S1PR1信号通路对心肌缺血再灌注损伤大鼠心肌炎症的影响

目的探讨麦冬皂苷D调节鞘氨醇激酶1(SphK1)/1-磷酸鞘氨醇(S1P)/鞘氨醇1磷酸酯受体1(S1PR)通路对心肌缺血再灌注损伤(MIRI)大鼠心肌炎症的影响。方法将大鼠随机分为MIRI组、麦冬皂苷D组、SphK1激活剂(K6PC-5)组、麦冬皂苷D+K6PC-5组、假手术组,每组12只。除假手术组外,其它组大鼠均通过结扎冠状动脉左前降支法构建MIRI模型。建模成功后,立即给药处理,每日1次,持续2周。超声成像系统评估大鼠左心室射血分数(LVEF)、左心室分数缩短(LVFS)变化;HE染色检测心肌组织的病理;ELISA法检测心肌组织中肌酸激酶同工酶(CK-MB)、乳酸脱氢酶(LDH)、白细胞介素(IL)-1β、肿瘤坏死因子α(TNF-α)水平;TUNEL染色检测心肌组织的心肌细胞凋亡;免疫组化染色心肌组织中Bim、天冬氨酸特异性半胱氨酸蛋白酶-3(Caspase-3)阳性细胞数占比;Western Blot法检测心肌组织中S1P、SphK1、S1PR1蛋白水平。结果与假手术组比较,MIRI组大鼠心肌结构损伤、纤维排列紊乱、心肌细胞减少、细胞核固缩且有大量炎症细胞浸润;LVFS、LVEF降低(P<0.05);心肌组织中CK-MB、LDH、IL-1β、TNF-α水平,心肌细胞凋亡率,Bim、Caspase-3阳性细胞数占比及S1P、SphK1、S1PR1蛋白水平升高(P<0.05)。与MIRI组比较,麦冬皂苷D组大鼠心肌结构损伤、纤维排列紊乱、心肌细胞减少、细胞核固缩及有大量炎症细胞浸润现象有所缓解;LVFS、LVEF升高(P<0.05);心肌组织中CK-MB、LDH、IL-1β、TNF-α水平,心肌细胞凋亡率,Bim、Caspase-3阳性细胞数占比及S1P、SphK1、S1PR1蛋白水平降低(P<0.05)。K6PC-5逆转了麦冬皂苷D对MIRI大鼠心功能障碍、心肌炎症及心肌细胞凋亡的影响(P<0.05)。结论麦冬皂苷D抑制MIRI大鼠心肌炎症及心肌细胞凋亡的机制可能与抑制SphK1/S1P/S1PR1通路有关。

Detection of Pseudorabies Virus Antibodies in Human Encephalitis Cases

Pseudorabies virus(PRV),a veterinary pathogen that infects domestic animals as well as wild animals such as wild boar and feral swine,was recently reported to infect human and led to endophthalmitis and encephalitis.A retrospective seroepidemiologic survey was conducted using 1,335 serum samples collected from patients with encephalitis and ELISA positive rates were 12.16%,14.25%,and 6.52%in 2012,2013,and 2017,respectively.

Microarray-Based Detection and Differentiation of Virulent and Attenuated Pseudorabies Virus

DNA microchip used in this study was formed from miniature arrays of pseudorabies virus （PrV） gene-specific probes immobilized on a glass surface. Hybridization using DNA microchip （microarrays） was used for differentiation between virulent and attenuated PrV. The presence of four gene segments （gB, gD, gE~, and gE ） encoding conservative glycoprotein B （gB）, D （gD）, and E （gE） of PrV was monitored using multiplex PCR. The amplicons were labeled with Cy5 or Cy3 dyes followed by hybridization to the gene-specific capture probes on the microchip. The presence of gD and gB, gE~ gene fragments was shown in virulent （gE~ genotype） and attenuated PrV （gE genotype）, whereas gE- gene （deleted domain in gE gene） was demonstrated only in virulent, not in attenuated, virus. No cross-hybridization was observed when fluorescence labeled-PCR products of PrV were hybridized using capture probes of related viruses, such as porcine respiratory and reproductive syndrome virus （PRRSV）, porcine parvovirus （PPV）, Japanese encephalitis virus （JEV）, and porcine circovirus type 2 （PCV-2）. The assay was 10 times sensitive than gD gene-specific PCR. Overall, the results of this study suggested that the microarray might be very useful for detection and differentiation of virulent PrV from attenuated one.

基于准PR调节器的三电平单相逆变器分岔现象研究

以2H桥级联式三电平单相逆变器为研究对象,利用频闪映射方法建立逆变器数学模型,利用分岔图、折叠图分析该逆变器的非线性现象,确定其稳定工作范围,对深刻理解和认识2H桥级联式三电平单相逆变器工作稳定性具有一定的意义,为提高逆变器系统工作稳定性能的设计和调试提供依据。