2022-2023年山东省A(H1N1)pdm09流感病毒HA、NA基因变异特征分析

目的 了解山东省2022-2023流感监测年度分离的A(H1N1)pdm09亚型流感病毒血凝素(hemagglutinin,HA)和神经氨酸酶(neuraminidase,NA)基因的变异特征,为流感的防控提供科学依据。方法 从流感监测网络实验室分离的流感毒株中按地市随机选取14株A(H1N1)pdm09亚型流感毒株,以WHO推荐的当季疫苗株为参考进行全基因组测序,并采用荧光法开展神经氨酸酶抑制(neuraminidase inhibition,NI)实验以评估药物敏感性。结果 山东省2022-2023年度分离的A(H1N1)pdm09流感病毒属于6B.1A分支中的5a.2a进化簇,核苷酸序列比对分析显示,HA和NA基因与2021-2023年度北半球疫苗株A/Victoria/2570/2019的亲缘关系较为接近,同源性分别为98.5%~98.7%和98.8%~99.1%。氨基酸序列分析显示,HA蛋白有20个位点发生了氨基酸序列变异,并发现1株病毒可能发生抗原漂移,有3株病毒发生了HA蛋白糖基化位点的缺失。NA酶相关重要位点未发生变异。NI实验显示,所测流感毒株均对抗流感病毒药物敏感。结论 所监测毒株与疫苗株整体同源性很高,但氨基酸存在一定程度变异,今后有必要持续开展流感病毒基因变异特征监测以了解流感流行的风险,以及评价基因变异对流感疫苗和治疗药物效果的影响。

表达H9亚型禽流感病毒HA基因的重组火鸡疱疹病毒构建及应用

为构建表达H9亚型禽流感病毒HA基因的重组火鸡疱疹病毒(herpesvirusofturkey,HVT),以连续覆盖HVT全基因组的Fosmid文库为基础,利用Red/ET同源重组技术和Gateway LR克隆技术,将优化的携带Pec复合启动子的HA基因插入到HVT复制非必需区HVT053与HVT054位点处的95318~95319nt之间,获得了表达H9亚型禽流感病毒HA基因的重组HVT(rHVT-H9-HA株),并对构建的毒株进行鉴定。结果显示,成功构建了含有HA基因的入门质粒pEntr-HA,通过Gateway克隆的LR反应将含有HA基因的表达盒转移到黏粒pFosC DEST的第53和54号基因之间形成pFosC HA;提取5个黏粒后,转染次代CEF细胞获得拯救重组病毒rHVT-H9-HA株。连续传代和动物试验结果表明,rHVT-H9-HA株毒价高,遗传稳定,可以克服母源抗体干扰,免疫持续期长,能够提供针对H9亚型禽流感的保护;同时也实现了一针防两病,效果明显优于灭活疫苗。本研究为H9亚型禽流感病毒重组HVT活载体疫苗的研制提供了技术支撑。

Sequence Analysis of HA Genes from Three H9N2 Subtype Avian Influenza Viruses

[ Objective] The study aimed to understand the genetic characters of H9N2 subtype avian influenza viruses isolated in Belling area. [ Method] HA genes of three H9N2 subtype avian influenza viruses A/Chicken/Beijing/xu/00, A/Chicken/Beijing/bei/00 and A/Chicken/Beijing/ liu/00 were amplified by RT-PCR and then sequenced. [ Result] The results of phylogenetic analysis showed that A/Chicken/Beijing/xu/00, A/ Chicken/Beijing/bei/00 and A/Chicken/Beijing/liu/00 shared the nucleotide homologies of 84.8% （ Dk/HK/Y439/97 ） -98.0% （ Ck/GX17/00 ）, 85.1% （Dk/HK/Y439/97） - 99.1% （ Ck/GXl 7/00）, 90.7% （ Ck/BJ/3/01 ） - 99.1% （Ck/GX17/00） with the isolates from Hongkong and other are- as of Chinese Mainland respectively. At the same time, the analysis of amino acid indicated that the three isolates belonged to low pathogenic H9N2 isolates of avian origin. The 226^th amino acid of them were L （ Leu）, suggesting their high binding affinity to human cells. There were seven glyco- sylation sites in HA protein, five from HA1 and two from HA2. [ Cenclusien] By analysis at molecular level, it could be concluded that A/Chicken/ Beijing/xu/00, A/Chicken/Beijing/bei/00 and A/Chicken/Beijing/liu/00 were low pathogenic H9N2 isolates of avian origin.

Sequence Comparison and Analysis of HA Gene of Four H9N2 Avian Influenza Virus Isolates

[ Objective] To determine the HA gene sequences of four H9N2 Avian influenza virus （AIV） strains and carry out comparative analysis so as to understand the difference and variation pattern of each strain from the angle of molecular biology and to know the distribution and epidemic law of H9N2 AIV. [Method] One pair of primers was designed referring to HA gene sequences of H9N2 AIV. The HA genes of A/Chicken/Hebei/WD/98 （H9N2; WD98 for short）, A/Chicken/Hebei/ZD/04 （H9N2; ZD04 for short））, A/Chicken/Beijing/MY/06 （H9N2; MY06 for short） ）, and A/Chicken/Beijing/PG/08 （H9N2; PG08 for short）） were amplified, cloned and sequenced. Then the HA gene sequences of these strains were compared with that of 10 H9N2 AIV stains in GenBank. [Result] The ORF of HA genes of the four strains was 1 683 bp in size, encoding 516 amino acids. The HA gene sequences of the four strains, WD98, MY06, PG08, and ZD04, were 82.6% -95.1%, 83.0% -99.0%, 82.7% -95.5%, and 81.3% -95.7% homologous to that of the 10 H9N2 AIV stains, respectively. And the homology of amino acid was respectively 86.6% -96.3%, 86.6% -97.9%, 87.0% -97.1%, and 86.9% -97.3%. [ Conclusion] The HA gene has greatly high homology among different strains.

长春市2016—2020监测年度甲型H1N1流感病毒血凝素(HA)基因特征分析

目的分析长春市2016—2020年度甲型H1N1流感病毒血凝素(HA)基因特征,了解其变异情况及遗传进化特征。方法选取2016—2020年度甲型H1N1流感病毒分离株109株,PCR扩增HA基因并进行序列测定;利用生物信息学软件对分离株的HA基因进行进化和变异分析。结果长春市109株分离株与疫苗株A/California/07/2009的HA蛋白相比均有S84N、S162N和I216T共同的氨基酸位点变异,且有1株发生了HA蛋白D222N位点突变,提示此毒株可引起患者下呼吸道症状。109株病毒株的HA基因之间核苷酸同源性为96.9%~100%,氨基酸同源性为97.2%~100%。在进化树分析上,都属于6B.1大分支,并且随着时间的推移,HA在基因进化树上离早期疫苗株A/California/7/2009越来越远,同一年份里也有毒株位于不同的小分支内。结论长春市2016—2020年度甲型H1N1流感病毒血凝素(HA)基因在不断的变异中,应持续进行监测,为预防甲型H1N1流感大流行提供参考。

Sequence and phylogenetic analysis of hemagglutinin genes of H9N2 influenza viruses isolated from chicken in China from 2013 to 2015

H9N2 avian influenza virus（AIV） infection is a major problem in poultry industry worldwide. In this study, molecular characterizations and phylogenetic relationships of hemagglutinin（HA） gene sequences of H9N2 AIV of 5 Chinese isolates in 2014 recently available in Gen Bank, 3 widely used vaccine strains, and 52 novel isolates in China from 2013 to 2015 were analyzed. The homology analysis showed that the nucleotide sequences of HA gene of these recent Chinese H9N2 AIV isolates shared homologies from 94.1 to 99.9%. Phylogenetic analysis showed that all isolates belonged to AIV lineage h9.4.2.5. Fifty-six out of the 57 recent Chinese H9N2 AIV isolates had the motifs PSRSSR↓GLF at the cleavage sites within the HA protein, while one isolate PWH01 harbored LSRSSR↓GLF. Remarkably, all of the recent Chinese H9N2 AIV strains had the Q216 L substitution in the receptor binding site, which indicated that they had potential to infect humans. Most of recent Chinese H9N2 AIV isolates lost the potential N-linked glycosylation site at residues 200–202 compared with vaccine strains. This present study demonstrated that AIV lineage h9.4.2.5 was more predominant in China than other lineages as it harbored all the H9N2 AIV isolated between 2013 and 2015. Also we showed the importance of continuous surveillance of emerging H9N2 AIV in China and update of vaccine formulation accordingly in order to prevent and control H9N2 AIV.

HA Gene Variation Analysis of H9N2 Sub-type Avian Influenza Virus from Three Strains in Different Times

HA Gene of H9N2. sub-type avian influenza virus from three strains in different times was amplified, purified and then sequenced. The results of its sequence analysis showed that the whole length of the amplified HA Gene was 1 683 bp, encoding 560 amino acids. The amino acid sequence of three virulent strains at cleavage site was R-S-S-R, which was low-pathogenicity strain. According to the amino acid sequence of the isolated strains, there were 7 potential glycosylation sites, and the receptor-binding site was the specific sequence of the avian-derived influenza virus. Amino acids on the left edge of receptor-binding site were all NGQQG, while amino acids on the right edge of receptor-binding site were GTSKA. From the comparative sequence analysis of HA Gene from some referenced strains, the results indicated that nucleotide and amino acid homology between isolated strains and referenced strains was higher. Evolutionary tree analysis showed that three strains were all Eurasian species, and there was a close relationship with the representative strains of A / duck / Hong Kong/Y280/97.

Mutations in Hemagglutinin of H5N1 Influenza That Switch Receptor Specificity from Avian to Human Types

Researchers have been searching for molecular features that could make avian H5N1 influenza transmissible among people since the first report of human infections with this virus in 1997. A recent study surprisingly demonstrated that only five mutations, fewer than previously estimated, are needed to make avian H5N1 influenza transmissible between ferrets through the air, raising fears that a human pandemic is possible if this virus escapes from the lab. Of the five mutations found, four of them are located in the HA gene that is responsible for the viral entry into the host cells. A crucial step for avian influenza to go across the species boundary to infect humans is the switch of its receptor binding specificity from avian to human types. The first task of this study was to quantify the individual as well as the collective effect of the known HA mutations from the previous research on receptor binding selection. Our second task was to identify new combinations of HA mutations that could change the receptor binding preference of H5N1 from avian to human types. Our findings thus deepened our understanding of the previous research and also extended its results by discovering new combinations of mutations that could enhance the binding of avian H5N1 to human type receptors while reduce that to avian types.

H7N9亚型禽流感病毒HA基因mRNA的构建

H7N9亚型禽流感病毒(AIV)持续给家禽及人类健康造成威胁。为构建H7N9亚型AIV(简称H7N9 AIV)mRNA疫苗,本研究以AIV分离株A/chicken/Yunnan/SD024/2021(H7N9)(简称CK/YN/SD024/2021)的HA基因为目的基因、选择来自人β-球蛋白和非洲爪蟾β-球蛋白的不同编码基因序列作为HA基因的非翻译区(UTR),构建了中间转录质粒pGEM-YN和pXT7-YN,以2个质粒为模板通过体外转录制备了mRNA mH7-YN-pGEM和mH7-YN-pXT7;将2种mRNA转染HEK293T细胞,western blot鉴定结果显示2种mRNA转染的细胞均可检测到约为70 ku的HA蛋白条带和50 ku的HA1蛋白条带;通过间接免疫荧光试验(IFA)确定最适转染剂量和HEK293T细胞中HA蛋白的动态表达,结果显示,3μg mRNA转染106个细胞并于转染24 h后荧光信号强度均最强;将2种mRNA转染鸡胚成纤维细胞(CEF),均可通过IFA检测到HA蛋白的表达。以上结果表明,本研究正确构建了2种含H7N9 AIV HA基因的mRNA,且其均能够在HEK293T细胞和CEF中正确表达HA蛋白,3μg mRNA转染HEK293T细胞可获得最佳的蛋白表达水平,转染24 h后HA蛋白的表达水平达到最高。本研究基于UTR序列的差异首次正确构建了两种能在哺乳动物细胞和禽类细胞中高效表达H7N9 AIV HA蛋白的mRNA,为禽流感mRNA疫苗的研发和免疫效力评估奠定了良好的物质和技术基础。

Construction and Immunogenicity of a Recombinant Adenovirus Expressing the HA Gene of H5N1 Subtype Swine Influenza Virus

To construct a recombinant adenovirus shuttle plasmid pDC315-H5HA-EGFP,the HA gene of A/Swine/Fujian/1/2001(H5N1) was amplified by RT-PCR and then inserted into adenovirus shuttle plasmid pDC315.A replication-defective recombinant adenovirus expressing the HA gene(rAd-H5HA-EGFP) was generated by co-transfecting the recombinant shuttle plasmid pDC315-H5HA-EGFP and the genomic plasmid pBHGlox△E1,E3Cre in HEK293 cells.The recombinant adenovirus was confirmed by PCR,RT-PCR and Western blot assay.These results demonstrated that HA protein was properly expressed by the rAd-H5HA-EGFP in HEK293 cells and had natural biological activities.The TCID50 of the rAd-H5HA- EGFP was assessed to be 2.26×1010/mL after propagation and purification.Immunization of BALB/ c mice indicated that rAd-H5HA-EGFP induced HI antibodies and protected mice from replication of the challenge virus in their lungs.

14株H9N2亚型禽流感病毒分离株的HA和NA基因序列分析

为了解浙江省H9N2亚型禽流感病毒(AIV)血凝素(HA)和神经氨酸酶(NA)基因的分子特征和遗传变异情况,本试验对2012—2021年分离到的14株H9N2亚型AIV分离株进行HA和NA基因序列测定和分析。结果显示:14株分离株的HA和NA基因均属于Y280分支,HA核苷酸同源性为91.5%~99.4%,NA核苷酸同源性为89.0%~98.7%,其与疫苗株CK/SS/94、CK/F/98、CK/6/96和CK/1/00的HA核苷酸同源性为86.0%~91.1%。14株分离株HA蛋白裂解位点氨基酸组成均为RSSR↓GLF;受体结合位点主要表现为K141N、A142T、T155N、H183N和V190T突变,其中第226位和第228位全部为L和G,可与α-2,6唾液酸受体结合,具有感染人的特性;蛋白潜在糖基化位点均为6个,主要变异表现在第200~202位1个位点缺失和第295~297位1个位点增加;抗原相关位点主要表现为G82E、S137D、D145G、N159G、A160D、T192R和N193D突变,此外,有5株出现D160N突变。14株分离株NA蛋白存在6个潜在糖基化位点,其中1株发生N86H突变,缺失1个潜在糖基化位点;均出现第61~63位颈部氨基酸缺失。结果表明,浙江省H9N2亚型AIV流行毒株不断变异,与疫苗株存在抗原性差异,需加强病毒变异监控和新疫苗研发。

Measles Virus(Nepal Strain)Hemagglutinin Gene: Cloning,Complete Nucleotide Sequence Analysis and Expression in COS Cells

Hemagglutinin gene of Measles virus(Nepal strain) was amplified by RT PCR technique, cloned and sequenced by the dideoxy mediated chain termination method. The comparison to the standard strain(Edmonston strain) showed many important mutations. The homology of these two strains was 98.17%. Then H gene was cloned into expression vector pCD SRα296 and introduced into COS 7 cells by electroporation method. The expression and function of cloned H gene was checked by hemadsorption assays.

Development of Neural Network for BLSOM Clustering of HA Genes of Avian Influenza Viruses Isolated in Guangdong Province

A neural network classification method,and a batch-learning self-organizing map(BLSOM),was established using trinucleotide and tetranucleotide in the hemagglutinin gene sequences of 25 avian influenza viruses isolated in Guangdong Province. Statistical analysis and normalization of the fragment number were done and MATLAB function was used to simulate the human brain thinking for self-organizing learning. When the number of training steps was 100 and above,the strains could be successfully clustered. H_1,H_3,H_5,H_7 and H_9 subtype strains fell within different classes,respectively,and the HA gene cluster map of H_3N_2 and H_7N_9strains was quite similar,suggesting that these strains shared the same origin; H_5N_1 strain was quite different in different years; H_1N_1 and H_9N_2 strains could be clustered into one group,indicating the natural recombinant variation in the two kinds of viruses,thereby providing a reference for high-risk strain screening and traceability.

广东地区H9N2亚型禽流感病毒HA和NA基因生物学特征分析

【目的】监测广东地区H9N2亚型禽流感病毒(Avian Influenza Virus,AIV)的遗传变异和分子进化趋势,为我国H9N2亚型AIV的防控提供参考。【方法】对2022年广东地区3株H9N2亚型AIV的HA和NA基因进行扩增、克隆、测序,使用DNAStar、PhyloSuite软件进行序列拼接和比对,再运用MEGA、Megalign、NetNGlyc 1.0Server等软件,对其核苷酸和氨基酸序列进行遗传进化、核苷酸同源性分析,以及受体结合、蛋白活性、耐药性和糖基化等关键位点分析。【结果】系统发育树和核苷酸同源性分析结果显示,3株分离株的HA和NA基因分别属于h9.4.2.5分支和1分支,与早期毒株的核苷酸同源性分别为81.6%~91.7%和88.2%~91.2%,分别命名为h9.4.2.5c分支和1.2分支;核苷酸和氨基酸序列分析发现,HA裂解位点为PSRSSR↓GLF,受体结合位点产生I155T、H183N、A190T/V、T212I、Q226L、Q227M突变,糖基化位点产生218N非糖基化和新增313N糖基化突变;NA茎部缺失187~195位9个核苷酸(ACAGAGATA),导致缺失63~65位3个氨基酸(TEI);NA红细胞结合位点产生K/E/S368N、D369N突变,与NA蛋白活性,耐药性的相关位点E119、D151、R152、R224、E276、R292、R371均未发生突变。【结论】2022年广东地区分离的3株H9N2亚型AIV已经进化成新的亚群,部分突变可能增强了对哺乳动物的适应性,且其抗原性发生改变,但尚未获得对奥司他韦和扎那米韦等抗流感病毒药物的耐药性。

Cloning and Analysis of Chitinase Gene in Bacillus subtilis HAS

[Objective] The paper was to study the possible mechanism of chitinase gene. [Method] The chitinase gene with inhibitory effect against a variety of pathogenic fungi was cloned and analyzed in this study. [Result] The genome of HAS strain contained an ORF of 834 bp. The homology of coding protein corresponding to ORF with chitosanase [Bacillus subtilis subsp. subtilis str. 168](ref|NP_390566.1) was the highest of 98%(272/277).[Conclusion]Through the analysis of amino acid sequence and secondary structure of the protease, tertiary structure prediction and analysis, HAS strain may play a pivotal role in controlling Sporisorium scitaminea Syd.

H7亚型禽流感病毒HA蛋白在Sf9中的表达与纯化

【目的】真核表达H7亚型禽流感病毒(Avian influenza virus,AIV)HA蛋白,为进一步制备H7亚型HIV亚单位疫苗,评价其免疫原性提供基础。【方法】首先根据草地贪夜蛾卵巢细胞(Spodoptera frugiperda clone 9,Sf9)的密码子偏嗜性,优化并合成H7亚型AIV的HA序列,将其克隆至穿梭质粒pFastBac1中;接着将重组HA基因的杆状病毒质粒转染至Sf9中,通过间接免疫荧光和Westernblots试验鉴定重组病毒是否拯救成功;再通过SYBRgreen染料法荧光定量PCR试验,建立基于gp64基因的杆状病毒qPCR定量方法,筛选出在Sf9中表达HA重组蛋白的最佳感染复数和孵育时间;最后通过His镍株亲和纯化HA重组蛋白。【结果】表达H7亚型AIV HA蛋白的重组杆状病毒在Sf9盲传3代后,Sf9开始出现肿胀、脱落、死亡等细胞病变,表明重组杆状病毒拯救成功;通过间接免疫荧光和Western blots试验发现,Sf9内出现可与HA重组蛋白特异性结合的绿色荧光信号,特异性结合的HA重组蛋白条带大小约70 kD左右,与预期相符,且HA重组蛋白可与H7亚型AIV阳性血清反应,表明HA重组蛋白表达成功;以构建的pUC19-gp64质粒为标准,建立基于gp64基因的杆状病毒qPCR检测方法,该方法在1×103~1×108 copy/μL间呈现良好的线性关系,标准曲线的相关系数R2=0.993;利用qPCR检测方法对杆状病毒液滴度进行定量,并通过Western blots试验筛选HA蛋白表达的最佳感染复数和孵育时间,结果显示以10MOI的比例接种Sf9,孵育72h,蛋白表达效果最好;通过His镍株亲和纯化HA重组蛋白,蛋白浓度为0.268mg/mL,鸡红细胞凝集效价为4log2。【结论】本试验在Sf9中成功表达并纯化H7亚型AIVHA蛋白,并建立与之相应的杆状病毒荧光定量PCR检测方法,可为进一步评价H7亚单位疫苗的免疫原性提供参考。

2022年山东地区商品肉鸡15株H9N2亚型禽流感病毒HA基因的遗传演化分析

为了解2022年商品肉鸡H9N2亚型禽流感病毒在山东地区的流行情况,选取了15株分离鉴定的H9N2亚型禽流感毒株,对其HA基因进行序列测定和分子特征分析,并应用软件Mega6.0绘制HA基因进化树,进行遗传进化分析。结果表明,15株H9N2分离毒的HA裂解位点氨基酸均为RSSR/GLF,具有典型低致病性AIV HA基因的特征;其第234位氨基酸均为亮氨酸(L),因此就具有了结合人流感受体的分子特性。进化树分析表明,2022年山东地区15株H9N2流行毒株HA基因属于4.2.5分支,细分为近几年在中国鸡群中流行的4.2.5a和4.2.5.c亚分支。

利用Rde/ET技术构建表达H5亚型禽流感病毒HA基因的重组火鸡疱疹病毒

【目的】本研究以火鸡疱疹病毒(HVT)BAC分子克隆为平台,构建表达禽流感HA基因的重组火鸡疱疹病毒,以开发新型病毒活载体疫苗。【方法】利用Red/ET重组技术,经过两步法重组:第一步,用两端带有50bp大小左、右同源臂a和b的选择标记基因rpsL-neo表达盒替换HVT基因组US2区;第二步,用两端带有同样的50 bp左、右同源臂a和b的HA基因表达盒替换选择标记基因rpsL-neo表达盒。在含有氯霉素和链霉素双抗性的平板上筛选阳性克隆,经卡那霉素抗性反向筛选和PCR进一步鉴定,鉴定正确的克隆命名为pHVT-HA。提取并纯化pHVT-HA DNA,转染原代鸡胚成纤维细胞(CEF),以完成重组病毒的拯救。【结果】命名为pHVT-HA3的BAC克隆转染CEF后第4天,出现病毒噬斑,噬斑形态与野生型HVT相似,获得拯救的重组病毒,命名为rHVT-HA3,将重组病毒rHVT-HA3在CEF上连续传代培养,经PCR和间接免疫荧光检测表明,重组病毒在连续传代过程中仍能稳定表达HA蛋白。【结论】本研究以HVT BAC为平台,利用Red/ET重组技术,构建了表达禽流感A/Goose/Guangdong/3/96(H5N1)毒株的血凝素(HA)基因的重组火鸡疱疹病毒,为新型禽流感重组活载体疫苗开发奠定基础。

高效表达H9亚型禽流感病毒HA基因的重组鸡痘病毒的构建及免疫效力试验

将禽流感病毒血凝素 H9A基因克隆入插入载体 p FG11S中 ,通过酶切鉴定获得了正向转移载体 p FG11SHA;将其与禽痘病毒疫苗株 (w FPV)共转染鸡成纤维细胞 (CEF) ,通过蓝白斑筛选纯化得到重组病毒 r FPV- Ps- HA;以间接免疫荧光法证实 HA基因得到了表达。将该病毒经颈部皮下免疫 1日龄 SPF鸡 ,免疫后 15 d以 H9亚型禽流感病毒 F株翅静脉攻毒 ,攻毒后第 5天采集泄殖腔棉拭子样品进行病毒分离。将此重组病毒与以痘苗病毒 P7.5启动子表达相同基因的重组病毒 r FPV- P7.5 - HA作比较 ,结果表明 ,r FPV- Ps- HA相对于 r FPV- P7.5 - HA明显抑制了病毒的排出 ;攻毒后第 2、5、7、9、11天分别对 r FPV- Ps- HA、油乳剂灭活苗免疫鸡进行泄殖腔、气管排毒规律的检测 ,发现疫苗组均能很好地抑制排毒 。

禽流感HA基因疫苗脂质体的制备及其理化性质

用改良的逆相蒸发法制备了Ｈ７亚型禽流感保护性抗原血凝素（ＨＡ）基因重组质粒ｐＳＶＨ７脂质体。电镜观察表明，该脂质体多呈球形的单层或多层结构，脂质体粒径分布均匀，粒径范围２０～７００ｎｍ，平均粒径１６３ｎｍ，主要粒径分布位于５０～２００ｎｍ（８４．８０％）。重组质粒ＤＮＡ在脂质体的制备过程中保持了稳定性，并能抵抗ＤＮＡ酶的水解破坏作用。吸收光谱表明，在２４８ｎｍ及２６８ｎｍ处脂质体有２个特征吸收峰，ＤＮＡ的存在不改变吸收峰的位置，但能增加吸收峰的强度。