Phylogenetic analysis of the haemagglutinin gene of canine distemper virus strains detected from breeding foxes,raccoon dogs and minks in China

Canine distemper virus (CDV) infects a variety of carnivores, including wild and domestic Canidae. Genetic/antigenic heterogeneity has been observed among the various CDV strains, notably in the haemagglutinin (H) gene, that appears as a good target to gather epidemiological information. Based on sequence analysis of the H gene, wild-type CDV strains cluster into distinct geographic lineages (genotypes), irrespective of the species of isolation. The sequence of the H gene of 28 CDV strains detected from both vaccinated and non-vaccinated breeding foxes, raccoon dogs and minks from different geographical areas of China during the years 2004–2008 was determined. All the CDV strains but two (strains HL and HLJ2) were characterized as Asia-1 genotype and were highly similar to each other (96.2–99.7% at the amino acid [aa] level) and to other Asia-1 strains (96.1–99.5% aa) previously detected in China. The CDV strains HL and HLJ2 were both collected from foxes in Heilongjiang province in 2005. Strain HL resembled CDVs of the Arctic genotype (GR88-like) and displayed high aa identity (98.0%) to the Chinese canine strain Liu. By converse, strain HLJ2 was barely related to CDVs of the Asia-2 genotype (88.7–90.3% aa identity), and could represent a novel CDV genotype, tentatively proposed as Asia-3. These results suggest that at least three different CDV genotypes, distantly related (81.8–91.6% aa identity) to the vaccine strains, Onderstepoort-like (America-1 genotype), are currently circulating in breeding foxes, raccoon dogs and minks in China, and that the genotype Asia-1 is predominant. Whether the diversity between wild-type CDVs and the vaccine strains may affect, to some extent, the efficacy of the vaccines deserves further investigations.     

The Establishment of AS-PCR Method to Distinguish Canine Distemper Asia-I Type Wild Strains and Vaccine Strains

Canine distemper (CD) is a contagious disease, which can damage the immune system, respiratory system, digestive system, and even nervous system, leading to systemic pathological changes, and has a huge threat to pet dogs, fur animals, etc. At present, the commonly used colloidal gold test cannot effectively distinguish vaccine immunity from animal natural infection. To establish an efficient and accurate detection method for identifying wild strains and vaccine strains of canine distemper virus(CDV), the whole genome of six canine distemper wild strains isolated from dogs and three widely used CDV vaccine strains collected from Wuhan area were sequenced. After comparing and analyzing the amino acid and the base sequences, the H gene was determined as the target gene for AS-PCR primer design. By genotyping the H gene, it was found that the prevalent CDVs in Wuhan were all Asia-Ⅰ, while the vaccine strain Y2 was America-I, and the vaccine strains Y1 and Y3 were both America-Ⅱ. Comparing the CDV-H gene sequences of 179 Asia-Ⅰtypes (6 wild-type strain samples + 173 GenBank Asia-Ⅰtype stains) and 3 vaccine strains, using AS-PCR technology (3'mismatch) to design a pair of primers. It can effectively distinguish CDV Asia-I wild strain and vaccine strain. The upstream primer sequence is 5'-TTAATATAATAATGACAGTG-3', and the downstream primer sequence is 5'-CCTCAAGGGGCACA-3'. The results showed that the primer had a strong specificity and the wild strains could amplify an 894 bp fragment, while the vaccine strains could not. There are 9 more regular bases (amino acids) variation sites in H gene of wild strain, and the 277th amino acids of all vaccine strains are Asparagine. These mutations may lead to an increase in N-glycosylation sites, which will have an impact on the virulence of canine distemper virus vaccine strains. The AS-PCR method established in this study can effectively distinguish the canine distemper vaccine and Asia-Ⅰwild strains.     

区分犬瘟热病毒Asia-Ⅰ型野毒株及疫苗株的AS-PCR方法

犬瘟热是一种接触性传染病,可侵害免疫系统、呼吸系统、消化系统,甚至神经系统,导致全身性的病理变化,对宠物犬、毛皮动物等存在巨大威胁。目前常用的胶体金检测法不能有效区分疫苗免疫与动物自然感染。为建立一种高效准确的鉴别犬瘟热病毒野毒株和疫苗株的检测方法,本试验对从武汉地区收集已确诊犬瘟热的6只犬分离得到的野毒株以及3株广泛使用的CDV疫苗株进行全基因组测序,从氨基酸水平和碱基水平比对分析后,确定H基因为AS-PCR引物设计的靶基因。通过对H基因进行分型,发现武汉地区流行的CDV均为Asia-Ⅰ型,而疫苗株Y2为America-I型,疫苗株Y1和Y3均为America-Ⅱ型。对比179株Asia-Ⅰ型（6株野毒株样品+173株GenBank Asia-Ⅰ型）与3株疫苗株的CDV-H基因序列,采用AS-PCR技术（3'端错配）设计出1对能有效区分犬瘟热Asia-Ⅰ型野毒株和疫苗株的特异性引物,上游引物序列为5'-TTAAATGATAATGACATAGTG-3',下游引物序列为5'-CCTGGCAAGGCAAGA-3'。结果显示该引物有较强的特异性,6株样品野毒株均可扩增出长894 bp的片段,疫苗株不能扩增,且野毒株的H基因上存在9个较为规律的碱基（氨基酸）变异位点,而疫苗株在第277位氨基酸上均为天冬酰胺,这些变异可能导致N-糖基化位点的增加,从而对犬瘟热病毒疫苗株的毒力产生影响。本研究建立的AS-PCR方法能有效区分犬瘟热疫苗和Asia-Ⅰ型野毒株。     

基于H蛋白基因的犬瘟热病毒遗传变异分析

犬瘟热是犬瘟热病毒(Canine distemper virus,CDV)感染犬和其他食肉动物造成的多发性、致死性传染病,本文从分子水平上探讨CDV遗传进化特性、变异情况与流行规律之间的关系.通过收集2002-2010年在中国地区分离的14株CDV野毒株、2006-2007年在全球各地分离的12株CDV野毒株以及从不同宿主分离的12株CDV野毒株和4株疫苗株,将其分为4组,将前3组野毒株分别与国内外正在使用的4株疫苗株的H基因进行遗传变异分析.分析发现,CDV野毒株与疫苗株间H蛋白基因的核苷酸相似性为86.2％～92.1％,其氨基酸相似性为89.1％～91.9％;H基因的584位的天冬酰胺糖基化位点是Asia-Ⅰ型CDV所特有的;H蛋白3555区域的非同义氨基酸替换概率较高.作者推测H蛋白抗原变异可能造成弱毒疫苗免疫效力降低,不能为某些CDV株的感染提供完全有效的保护.     

犬瘟热病毒SH202003株全基因组序列分析

为了解上海地区犬瘟热病毒（Canine distemper virus，CDV）遗传变异情况，本研究采用首尾重叠的11对特异性引物，对CDV上海株SH202003进行RT-PCR扩增，将扩增片段进行反复测序，序列拼接后最终获得了SH202003株全基因组序列，应用Lasergene 7.0和Mega 6.0软件对全基因及H基因进行序列分析，并构建系统进化树。结果显示，SH202003株基因组全长为15 690 bp，编码6种结构蛋白（N、P、M、F、H和L），H和L基因间隔序列为CUA，L和5'端尾随序列为CAA，与Hebei株核苷酸和氨基酸相似性最高，达到98.6%和96.6%，与疫苗株核苷酸相似性在92.2%~94.3%，氨基酸相似性只有82.7%~87.0%；全基因进化树中，SH202003株与流行野毒株在同一分支，与疫苗株在不同的分支；H基因同样与Hebei株亲缘关系最近，核苷酸和氨基酸相似性分别为98.7%和99.5%，与疫苗株Snyder Hill、CDV3、Convac及Onderstepoort亲缘关系较远；SH202003株处于Asia-1型分支，属于Asia-1型强毒株；SH202003株具有9个潜在N-糖基化位点，与强毒株Hebei株一致。研究表明，上海株SH202003属于CDV强毒株，为Asia-1型，其H基因序列相对保守，具有9个潜在N-糖基化位点，但是全基因序列存在较多突变，与疫苗株的匹配度较差，可能是免疫犬依然发生犬瘟热的主要原因。     

小熊猫源犬瘟热病毒株H、F基因的克隆及序列分析

为了解1株圈养小熊猫源犬瘟热病毒（CDV）GD-1的遗传变异情况,通过RT-PCR方法对该株CDV进行H、F基因的克隆、测序及序列分析。结果显示：该分离株的H基因序列与GenBank中丹麦报道的登录号为GU266280的犬源CDV毒株的核苷酸序列相似性最高,为96%;F基因序列与巴西报道的登录号为KY057355的犬源CDV的核苷酸序列相似性最高,为95.7%。下载CDV代表毒株序列进行遗传演化、氨基酸序列比对及分子特征分析。结果显示：H蛋白共有8个潜在的N-糖基化位点,分别位于19、149、309、391、422、456、587、603位点;H蛋白的SLAM受体结合位点氨基酸序列与欧亚野生型毒株一致,与疫苗株相比,530、549位氨基酸不同,与其他CDV参考毒株H蛋白相比还存在24、41等9处氨基酸位点发生明显变异,与标准强毒株A75/17的氨基酸相似性为95.2%,与Onderstepoort、Convac等5株疫苗株的氨基酸序列相似性为88.2%~89.3%;F蛋白共有6个N-糖基化位点,分别位于62、108、141、173、179、517位,与Onderstepoort等疫苗株氨基酸相似性为89.1%~89.7%;与其他参考毒株相比还存在115、130等11处氨基酸发生变异;构建基于H、F基因的遗传进化树,结果显示：该毒株位于Asia-4型的一个小的进化分支,这与目前我国流行毒株主要位于Asia-1型存在明显不同。本研究首次报道了小熊猫源的Asia-4基因型CDV野毒株,并对毒株的H及F基因进行了序列分析,对于了解我国CDV流行株的遗传变异情况、流行病学调查、疾病防控及疫苗研发等具有重要意义。     

北京地区犬瘟热病毒分离株H基因的分型

根据发表的犬瘟热病毒(CDV)参考毒株Onderstepoort的序列设计了一对引物,以感染犬瘟热病毒的犬的粪便总RNA为模板,RT-PCR扩增出17株CDV的H全基因1877bp的片段,将这个片段连接到pGEM-Teasy载体上,经酶切鉴定得到阳性克隆,将阳性质粒进行序列测定,并与国内外毒株进行同源性比较和系统发育分析,结果显示17株均为Asia-1型。北京地区流行的毒株主要是America-1型和Asia-1型,其中2007年主要流行America-1(疫苗型),而2008年主要是Asia-1型。     

Heterogeneity within the hemagglutinin genes of canine distemper virus (CDV) strains detected in Italy

Canine distemper virus (CDV) is a highly contagious viral pathogen causing lethal disease in dogs and other mammalians. A high degree of genetic variation is found between recent CDV strains and the old CDV isolates used in the vaccines and such genetic variation is regarded as a possible cause of the increasing number of CDV-related diseases in dogs. The H gene shows the greatest extent of genetic variation that allows for distinction of various lineages, according to a geographical pattern of distribution and irrespective of the species of identification. In the present study, hemagglutinin (H) genes obtained from field strains detected from clinical specimens of Italian dogs were analyzed genetically. Phylogenetic analysis revealed that a homogeneous group of CDV strains is widespread in Italian dogs, all which are included into the European lineage. Unexpectedly, strains 179/04 and 48/05 clustered along with CDVs of the Arctic lineage, the highest identity being to strain GR88 (98.0 and 98.4%aa, respectively). The full-length sequence of a red fox CDV strain, 207/00 was also determined and analyzed. The H protein of the fox CDV strain was unrelated to strains within the major European lineage. These results suggest that at least three different CDV lineages are present in Italy.     

CDV强毒BJ16B2株H基因在昆虫杆状病毒中的表达与鉴定

试验旨在获得具有天然构象且抗原性良好的犬瘟热病毒（canine distemper virus,CDV）强毒株的H蛋白。以分离的CDV强毒株BJ16B2为模板,RT-PCR特异扩增H基因,克隆至表达载体pFastBac^TM HTA上,酶切及测序鉴定正确后比对分析H基因同源性,并将重组质粒pFastBac^TMHTA-H转化大肠杆菌DH10Bac^TM感受态细胞,同源重组构建穿梭质粒rBacmid-H,将重组穿梭质粒转染Sf9昆虫细胞,拯救重组杆状病毒。利用IFA和Western blotting对获得的重组蛋白进行鉴定及抗原性分析。结果显示,重组质粒pFastBac^TMHTA-H酶切测序鉴定正确,该H基因属于Asia-1强毒株,与参考毒株的核苷酸和氨基酸同源性分别为89.8%~99.3%和89.6%~99.5%。在杆状病毒中所表达的H蛋白能与CDV阳性血清及His-tag抗体发生特异性反应,IFA鉴定能够产生特异性绿色荧光,且在68 ku左右出现蛋白条带,表明H蛋白成功表达且具有良好的反应原性。本研究获得了具有天然构象及良好抗原性的CDV重组H蛋白,为后续蛋白结构和抗原特性差异分析、单抗制备、CDV亚单位疫苗的开发奠定了基础。     

Phylogenetic analysis of Austrian canine distemper virus strains from clinical samples from dogs and wild carnivores

Austrian field cases of canine distemper (14 dogs, one badger [Meles meles] and one stone marten [Martes foina]) from 2002 to 2007 were investigated and the case histories were summarised briefly. Phylogenetic analysis of fusion (F) and haemagglutinin (H) gene sequences revealed different canine distemper virus (CDV) lineages circulating in Austria. The majority of CDV strains detected from 2002 to 2004 were well embedded in the European lineage. One Austrian canine sample detected in 2003, with a high similarity to Hungarian sequences from 2005 to 2006, could be assigned to the Arctic group (phocine distemper virus type 2-like). The two canine sequences from 2007 formed a clearly distinct group flanked by sequences detected previously in China and the USA on an intermediate position between the European wildlife and the Asia-1 cluster. The Austrian wildlife strains (2006 and 2007) could be assigned to the European wildlife group and were most closely related to, yet clearly different from, the 2007 canine samples. To elucidate the epidemiological role of Austrian wildlife in the transmission of the disease to dogs and vice versa, H protein residues related to receptor and host specificity (residues 530 and 549) were analysed. All samples showed the amino acids expected for their host of origin, with the exception of a canine sequence from 2007, which had an intermediate position between wildlife and canine viral strains. In the period investigated, canine strains circulating in Austria could be assigned to four different lineages reflecting both a high diversity and probably different origins of virus introduction to Austria in different years.     

检测和鉴别犬瘟热病毒强、弱毒株的复合反转录-套式聚合酶链式反应(RT-nPCR)的建立及初步应用

根据GenBank上登录的犬瘟热病毒（Canine distemper virus，CDV）基因组全序列，选择CDV强、弱毒株间有区别保守区设计了一对通用引物P1和P4，并在该对引物跨越区域的内部设计了CDV强毒株特异性引物P2及弱毒株特异性引物P3，用引物P1／P4进行RT—PCR，然后用引物P2／P3／P4进行复合套式PCR，建立了一种能区分CDV强、弱毒株的复合反转录-套式聚合酶链式反应（RT—nPCR）的鉴别诊断方法。应用该方法从CDV强、弱毒株的基因组中分别扩增出了大小为247bp和177bp的特异性片段，从两种病毒基因组混合物中扩增出了大小为247bp和177bp的两条特异性片段，与犬细小病毒、犬腺病毒、犬冠状病毒、狂犬病病毒、新城疫病毒的细胞培养物以及正常细胞对照组进行复合RT—nPCR扩增时均为阴性。对从黑龙江省和吉林省采集的20份疑似CDV病料进行的检测结果表明，有15份类似CDV强毒，5份类似CDV弱毒。本研究建立的复合RT—nPCR可以有效检测CDV感染，能够将强、弱毒株区分开，可用于临床快速检测、流行病学监测以及追踪疫苗免疫效果等。     

表达犬瘟热病毒H基因重组新城疫病毒的构建及其免疫原性研究

为研制安全、有效的新型犬瘟热疫苗,本研究利用新城疫病毒(NDV) LaSota弱毒疫苗株反向遗传操作系统,构建出表达犬瘟热病毒(CDV)弱毒疫苗株Rockborn-20/8血凝素(H)蛋白的重组病毒rLa-CDV-H,并对其生物学特性进行鉴定,评估其作为犬瘟热活载体疫苗的安全性和有效性.通过免疫荧光和western blot试验证明了CDV H蛋白的正确表达;重组病毒株保持了LaSota亲本株的低致病性和高滴度鸡胚生长特性;重组病毒rLa-CDV-H接种12周龄比格犬后,可以诱导显著的CDV中和抗体反应.本研究表明重组病毒rLa-CDV-H具有作为犬瘟热重组病毒活载体疫苗的潜力.     

犬瘟热病毒小熊猫株H、F和N基因的克隆及表达

根据GenBank中发表的犬瘟热病毒（CDV）的核苷酸序列，设计并合成了扩增CDVH、F和N基因的3对引物，经RT—PCR分别扩增获得了CDV小熊猫株（LP株）H、F和N基因，并对H、F及N基因进行了克隆和序列测定。序列分析表明，CDV LP株属于强毒谱系，与CDV流行株的亲缘关系近．H基因含有较多潜在的糖基化位点．F和N基因相对比较保守。将CDV LP株H、F和N基因克隆入真核表达栽体pVAX1的CMV启动子下游，构建了CDV基因疫苗表达载体pVAXLPH、pVAXLPF、pVAXLPN，体外转染BHK-21细胞．用间接ELISA方法检测到目的蛋白的表达。用构建的3个表达质粒免疫小鼠，从小鼠血清中检测到了抗CDV抗体．初步证实用CDVH、F和N基因作为核酸疫苗免疫动物，可以激活机体的免疫应答。     

水貂犬瘟热病毒分离鉴定及其H基因序列分析

为了解山东地区水貂犬瘟热病毒(CDV)遗传变异特征,采集水貂养殖场的发病水貂病料,通过RT-PCR鉴定为CDV阳性,将阳性病料接种Vero/Dog SLAM细胞进行病毒分离,通过间接免疫荧光、电镜负染、测序等方法鉴定,得到4株犬瘟热病毒,分别命名为WD1株、WD2株、WX1株和WX2株。分离株H基因测序结果显示,WD1株、WD2株、WX1株均为Asia-Ⅰ型,其中WD1和WD2与近几年仅在水貂和狐狸养殖场流行的新犬瘟热毒株核苷酸和氨基酸序列同源性分别为97.5%~99.2%和97%~99%;WX-1型与国内犬源HL001株的同源性最高,核苷酸和氨基酸序列同源性分别为99.6%和99.5%;WX2与疫苗株同属于一个分支,与疫苗毒Lederle株核苷酸和氨基酸序列同源性高达99.5%和98.8%。结果表明,水貂养殖场存在多株犬瘟热病毒混合感染的情况,提醒养殖场应注意防控,该结果也为犬瘟热病毒分子流行病学积累了资料。     

Identification of a new genotype of canine distemper virus circulating in America

Canine Distemper is a highly contagious viral systemic disease that affects a wide variety of terrestrial carnivores. Canine Distemper virus (CDV) appears genetically heterogeneous, markedly in the hemagglutinin protein (H), showing geographic patterns of diversification that are useful to monitor CDV molecular epidemiology. In Mexico the activity of canine distemper remains high in dogs, likely because vaccine prophylaxis coverage in canine population is under the levels required to control effectively the disease. By phylogenetic analysis based on the nucleoprotein (N) and on the H genes, Mexican CDV strains collected between 2007 and 2010 were distinguished into several genovariants, all which constituted a unique group, clearly distinct from field and vaccine strains circulating worldwide, but resembling a CDV strain, 19876, identified in Missouri, USA, 2004, that was genetically unrelated to other North-American CDV strains. Gathering information on the genetic heterogeneity of CDV on a global scale appears pivotal in order to investigate the origin and modalities of introduction of unusual/novel CDV strains, as well as to understand if vaccine breakthroughs or disease epidemics may be somewhat related to genetic/antigenic or biological differences between field and vaccine strains.     

应用流式细胞术研究犬瘟热病毒感染细胞的凋亡

用犬瘟热病毒 ( CDV) 2种不同毒株感染非洲绿猴肾细胞 ( Vero) ,用流式细胞术分析了病毒诱导的感染细胞的凋亡。结果发现 ,2种毒株感染引起的细胞病变类型不同 ,分为圆缩型与合胞体型 ;2种毒株均可诱导感染细胞凋亡 ,但毒株间的凋亡细胞比例存在差异 ,即产生合胞体型细胞病变的毒株凋亡出现较晚 ,凋亡细胞比例显著低于产生圆缩型细胞病变的毒株 ( P<0 .0 1 )。结果提示 ,不同毒株导致细胞死亡的机制可能不同     

水貂、狐狸和貉源犬瘟热病毒F蛋白信号肽区基因克隆及遗传变异分析

为了解近年来犬瘟热病毒(canine distemper virus,CDV)在中国毛皮动物主要养殖区的流行情况及遗传变异情况,本试验于2012-2014年从山东、河北、辽宁收集疑似犬瘟热的水貂、狐狸和貉病料,经犬瘟热抗原检测试纸条检测和RT-PCR检测为阳性后,克隆测序了15株CDV F蛋白信号区(Fsp)基因序列.序列分析结果显示,15株CDV野毒株Fsp基因核苷酸序列和氨基酸序列的相似性均为93.6%~100.0%,与疫苗株相似性为80.7%~81.7%.基因系统进化分析结果显示,15株野毒株均属于中国当前流行的Asia-1基因型.氨基酸序列比对分析结果显示,Fsp蛋白在氨基酸3-14、16-37、47-67位等处存在高变异.通过对当前流行CDV野毒株Fsp基因序列分析,结果表明该Fsp基因区具有较高的变异率,可作为CDV基因分型的依据,同时本试验结果为毛皮动物犬瘟热的防控提供了参考依据.     

鉴别犬瘟热病毒疫苗株和野毒株RT—PCR—RFLP方法的建立及应用

根据Onderstepoort株H基因序列,设计1对引物建立RT-PCR-RFLP检测方法,对不同宿主来源的疑似犬瘟热临床样品进行检测,并对检出的犬瘟热病毒野毒山东株PCR产物进行克隆和序列分析,验证RT—PCR—RFLP检测方法。结果RT—PCR扩增片段为1921bp,产物经RFLP分析,野毒株的PCR产物能被NdeI酶切为1282、345和294bp3个片段,弱毒疫苗株则不能被切开;病毒RNA的最小检出量为2．15ng。临床检测共检出19份样品为犬瘟热阳性,其中15份为野毒株感染,其H基因编码区全长为1824bp,均在1279和1543处有NdeI酶切位点,推导氨基酸与野毒株的同源性在92．9％～96．9％,与疫苗株的同源性在89．0％～90．8％,进化树分析显示这些毒株在基因型上属于Asia-1型,为野毒株谱系。该方法的建立为临床上犬瘟热病毒的鉴别检测和诊断提供了依据。     

Propagation of Asian isolates of canine distemper virus (CDV) in hamster cell lines

Backgrounds

The aim of this study was to confirm the propagation of various canine distemper viruses (CDV) in hamster cell lines of HmLu and BHK, since only a little is known about the possibility of propagation of CDV in rodent cells irrespective of their epidemiological importance.

Methods

The growth of CDV in hamster cell lines was monitored by titration using Vero.dogSLAMtag (Vero-DST) cells that had been proven to be susceptible to almost all field isolates of CDV, with the preparations of cell-free and cell-associated virus from the cultures infected with recent Asian isolates of CDV (13 strains) and by observing the development of cytopathic effect (CPE) in infected cultures of hamster cell lines.

Results

Eleven of 13 strains grew in HmLu cells, and 12 of 13 strains grew in BHK cells with apparent CPE of cell fusion in the late stage of infection. Two strains and a strain of Asia 1 group could not grow in HmLu cells and BHK cells, respectively.

Conclusion

The present study demonstrates at the first time that hamster cell lines can propagate the majority of Asian field isolates of CDV. The usage of two hamster cell lines suggested to be useful to characterize the field isolates biologically.     

水貂犬瘟热Vero细胞活疫苗（CDV3-CL株,悬浮培养）安全性评价

为考察新研制的水貂犬瘟热Vero细胞活疫苗(CDV3-CL株,悬浮培养)的安全性,分别以一次单剂量(1头份)、单剂量重复和一次超剂量(10头份)接种动物,对疫苗进行全方位安全性评价,试验动物涉及水貂幼崽、育成水貂以及妊娠水貂等,重点观察注射动物的体温、食欲,生产性能是否发生改变、注射部位是否出现炎症反应以及实验动物接种部位组织病变等,连续观察15d,结果发现,实验动物没有发生炎症反应,动物体温变化也处于正常范围内,证明疫苗是安全的,从而为疫苗的推广奠定基础。