Evaluation of Germplasm Using SSR Markers of Functional Genes in Rice

16 SSR (Simple sequence repeats) primers of functional genes in rice were used to detect genetic diversity among 23 accessions of rice germplasm from 5 countries in the world. The average number of alleles per SSR locus was 5.2 with a range from 2 to 10. Genetic similarities among the 23 rice accessions ranged from 0.13 to 0.64. UPGMA cluster analysis showed that the 23 rice accessions could be classified into two distinct classes at similarities with a coefficient of 0.13. The Japonicas from Brazil, Japan and China were classified into Class I, along with upland rice from Brazil. The Indicas from Pakistan and Korea were classified into Class Ⅱ. Consequently, the function of genes SSR markers could be used as a useful tool for measuring genetic diversity, assigning rice to geographical distribution, ecotype, and pedigree relationship.     

Genetic diversity analysis of Brassica oleracea L. by SSR

SSR analysis on genetic diversity of 30 samples was carried out.Five primers selected from 36 primers were used to amplify 30 samples in this experiment,PCR products were separated by 6% polyacrylamide gel electrophoresis,silver staining and photographed.The results of SSR were analyzed by UPGMA clustering.The results showed that a total of 21 gene alleles were detected by 5 SSR primers.The number of alleles ranged from 2 to 5 with an average of 4.2.PIC range was 0.257-0.921,with an average of 0.543.The average coefficient of genetic similarity of SSR markers among materials was 0.432.Some of cabbage cultivars in the experiment were divided into four groups except cultivars which come from Japan.     

Development of SSR Markers for a Phytopathogenic Fungus,Blumeria graminis f.sp.tritici,Using a FIASCO Protocol

Simple sequence repeats （SSR） have been widely used as molecular markers due to their abundance and high polymorphism, However, up to now, the SSR markers had not been developed in the obligate biotrophic phytopathogenic fungus, Blumeria graminis f.sp. tritici. From （AC）10 and （AG）10 enriched genomic libraries for Bgt, 25 primer pairs were designed using the FIASCO （fast isolation by AFLP of sequences containing repeats） protocol. Five primer pairs exhibited polymorphism with allelic diversity from two to seven alleles and produced 29 alleles in a survey of 90 isolates collected from six provinces （cities） in China, while the others displayed monomorphic. Levels of observed heterozygosity ranged from 0.000-0.044 （mean 0.025） and expected heterozygosity ranged from 0.297-0.816 （mean 0.538）. These molecular markers provide a novel source to genetic diversity assays and to genetic and physical mapping ofBgt. SSR markers of Bgt need to be further explored.     

Identification and Analysis of Genetic Diversity Structure Within Pisum Genus Based on Microsatellite Markers

To assesse the genetic diversity among wild and cultivated accessions of 8 taxonomic groups in 2 species, and 5 subspecies under Pisum genus, and to analyze population structure and their genetic relationships among various groups of taxonomy, the study tried to verify the fitness of traditionally botanical taxonomic system under Pisum genus and to provide essential information for the exploration and utilization of wild relatives of pea genetic resources. 197 Pisum accessions from 62 counties of 5 continents were employed for SSR analysis using 21 polymorphic primer pairs in this study. Except for cultivated field pea Pisum sativum ssp. sativum var. sativum （94 genotypes）, also included were wild relative genotypes that were classified as belonging to P. fulvum, P. sativum ssp.abyssinicum, P. sativum ssp. asiaticum, P. sativum ssp. transcaucasicum, P. sativum ssp. elatius var. elatius, P. sativum ssp. elatius var. pumilio and P. sativum ssp. sativum var. arvense （103 genotypes）. The PCA analyses and 3-dimension PCA graphs were conducted and drawn by NTSYSpc 2.2d statistical package. Nei78 genetic distances among groups of genetic resources were calculated, and cluster analysis using UPGMA method was carried out by using Popgene V1.32 statistical package, the dendrogram was drawn by MEGA3.1 statistical package. Allelic statistics were carried out by Popgene V1.32. The significance test between groups of genotypes was carried out by Fstat V2.9.3.2 statistical package. 104 polymorphic bands were amplified using 21 SSR primer pairs with unambiguous unique polymorphic bands. 4.95 alleles were detected by each SSR primer pair in average, of which 65.56% were effective alleles for diversity. PSAD270, PSAC58, PSAA18, PSAC75, PSAA175 and PSAB72 were the most effective SSR pairs. SSR alleles were uniformly distributed among botanical taxon units under Pisum genus, but significant difference appeared in most pairwise comparisons for genetic diversity between taxon unit based groups of genetic resources. Genetic diversity level of wild species P. fulvum was much lower than the cultivated species P. sativum. Under species P. sativum, P. sativum ssp. sativum var. sativum and P. sativum ssp. asiaticum were the highest in gentic diversity, followed by P. sativum ssp. elatius var. elatius and P. sativum ssp. transcaucasicum, P. sativum ssp. elatius var. pumilio, P. sativum ssp. sativum vat. arvense and P. sativum ssp. abyssinicum were the lowest. Four gene pool clusters were detected under Pisum genus by using PCA analysis. Gene pool ＂fulvum＂ mainly consisted of wild species Pisum fulvum, gene pool ＂abyssinicum＂ mainly consisted of P. sativum ssp. abyssinicum, and gene pool ＂arvense＂ mainly consisted of P. sativum ssp. sativum var. arvense. While gene pool ＂sativum＂ were composed by 5 botanical taxon units, they are P. sativum ssp. asiaticum, P. sativum ssp. elatius var. elatius, P. sativum ssp. transcaucasicum, P. sativum ssp. elatius var. pumilio and P. sativum ssp. sativum var. sativum. ＂sativum＂ gene pool constructed the primary gene pool of cultivated genetic resources; ＂fulvum＂ gene pool, ＂abyssinicum＂ gene pool and ＂arvense＂ gene pool together constructed the secondary gene pool of cultivated genetic resources. Pairwise Nei78 genetic distance among botanical taxon based groups of pea genetic resources ranged from 7.531 to 35.956, 3 large cluster groups were identified based on the UPGMA dendrogram. Group Ⅰ equals to ＂sativum＂ and ＂arvense＂ gene pools, Group Ⅱ equals to ＂abyssinicum＂ gene pool, and Group Ⅲ equals to ＂fulvum＂ gene pool. The UPGMA clustering results generally supporting the PCA clusting results. There were significant differences among most botanical groups under Pisum genus, with clear separation of four gene pools for genetic diversity structure. The research results partially support the traditional botanical taxonomy under Pisum genus, and pointed out its advantage and shortcoming. In order to broaden the genetic bases of pea varieties, the genetic potentials in the four gene pools should be thoroughly exploited.     

Genetic Diversity Analysis Among Populations of Mink from China by Inter-simple Sequence Repeat （ISSR） Markers

Inter-simple Sequence Repeat （ISSR） analysis was applied to assess the genetic diversity within and among five populations of mink from Liaoning Province. A total of 20 primers were screened, five selected primers produced 35 discernible bands, with 30 （85.71%） being polymorphic, indicating high genetic diversity at the species level. The highest genetic diversity was observed in the brown mink population, whereas the lowest diversity was found in the standard-pitchy mink population. Based on genetic distance （1972）, a dendrogram was constructed by using UPGMA algorithm, and five populations were divided into two major groups. Group I consisted of only the standard-pitchy mink population, and Group II included other four populations, in Group II, sapphire mink was close to brown mink population. The results of genetic differentiation indicated that the genetic differentiation degree between populations was lower and the genetic variation primarily came from within populations. This paper showed that ISSR technique was a reliable tool that could be used to study genetic diversity in the mink.     

Analysis of SSR Fingerprints in Introduced Silkworm Germplasm Resources

Thirty-five SSR markers were used to construct 96 silkworm races fingerprint. All the SSR markers were polymorphic and unambiguously separated silkworm strains from each other. A total of 467 alleles were detected with a mean value of 13.34 alleles/locus （range 3-28）. The mean polymorphism index content （PIC） was 0.71 （range 0.299-0.919）. UPGMA cluster analysis of Nei＇s genetic distance grouped silkworm strains on the basis of their origin. The results indicated that SSR markers are efficient tools for fingerprinting cultivars and conducting genetic diversity studies in the silkworm.     

Analysis of Genetic Diversity in Natural Populations of huashanica Keng Using Microsatellite （SSR） Markers

Psathyrostachys huashanica Keng is endemic to China and only distributed in Huashan Mountain in Shaanxi Province, China. In this study, 15 P. huashanica populations consisting of 450 individuals sampled across their main distribution were investigated by using the simple sequence repeats （SSRs） markers. A total of 184 alleles were detected on 24 SSR loci, and the number of alleles on each locus ranged from 2 to15, with an average of 7.667. The total gene diversity （HT= 0.683） and the coefficient of population differentiation （GST = 0.125） showed that P. huashanica had a relatively high level of genetic variation, and the genetic variation was mainly distributed within the populations. The gene flow among the populations of P. huashanica （Nm = 1.750） was much less than that of the common anemophytes （Nm = 5.24）. Correlation analysis demonstrated that the number of alleles as well as genetic diversity of the five populations of Huangpu valley decreased along with the increase of altitudes, but the correlation was not significant. Implications of these results for future P. huashanica collection, evaluation and conservation were discussed.     

Analysis of the Genetic Diversity and Origin of Some Chinese Domestic Duck Breeds

Twelve fluorescence-labeled microsatellite markers were used to analyze the genetic diversity of 12 domestic duck breeds and 2 wild duck breeds to determine the relationship and origin of Chinese domestic duck breeds. Gene frequency, effective number of alleles （Ne）, expected heterozygosity （He）, polymorphism information contents （PIC）, inbreeding coefficient in population （Fis）, standard genetic distance （Ds）, and genetic distance （DA） were calculated by FSTAT and distance and phylogenetic analysis after the dates which were output from the Microsatellite-Toolkit software. Genetic distances between 12 domestic duck breeds and 2 wild duck breeds were analyzed by variance analysis. Unweighted pair group method with arithmetic mean （UPGMA） and phylogenetic trees used for cluster analysis were structured. The results indicated that 11 loci had medium- or high-level genetic diversity among the 12 loci, which could be efficiently used in the detection of the genetic parameters of each population. The values of He were 0.5414 to 0.7343, those of PIC proved similar, and those of Fis were 0.1101 to 0.3381 among all populations. All breeds were clustered into three groups by UPGMA phylogenetic trees. Banzui duck was clustered into a separate group. Differences of the DA were analysed by t-test. The results showed that difference in DA between the 12 domestic duck breeds and Lvtou duck and the Banzui duck were very significant （P〈0.01）, indicating that these 12 domestic duck breeds originated from Lvtou wild duck, but not Banzui duck.     

Genetic Relationships Among Chinese Maize OPVs Based on SSR Markers

Bulk-SSR method was used to analyze the genetic diversity of 44 open-pollinated varieties collected from Henan, Shandong, Shanxi, and Jilin provinces and Guangxi Zhuang Autonomous Region, China using 70 pairs of SSR primers. The purposes of this study were to (1) compare the genetic diversity among 44 Chinese maize open-pollinated varieties; (2) estimate the minimum number of alleles for construction of a stable dendrogram; and (3) trace the genetic relationships among local germplasm from different regions of China. In total, these 70 SSR primers yielded 292 alleles in 176 samples (4×44) analyzed. The number of alleles per locus was 4.17 on average and ranged from 2 to 8. The highest number of alleles per open-pollinated variety (55.25) was detected in Shanxi germplasm, which indicated that open-pollinated varieties from Shanxi possessed the largest genetic diversity among those from the five locations. The correlation coefficients between different genetic similarity matrices suggested that 200 alleles were sufficient for analysis of the genetic diversity of these 44 open-pollinated varieties. The cluster analysis showed that 44 open-pollinated varieties collected from three growing regions in China were accurately classified into three groups that were highly consistent with their geographic origins, and there is no correlation between GS and geographic distance in this study.     

Phylogenetic Relationships in Genus Arachis Based on SSR and AFLP Markers

Fourteen wild species of different sections in the genus Arachis and 24 accessions of the AABB allotetraploid A. hypogaea （cultivated peanut） from several countries which belong to different botanical varieties, were analyzed by SSR and AFLP marker systems. The assay-units per system needed to distinguish among all the tested accessions were at least five for SSR or two for AFLP. The genetic distance detected by the SSR markers ranged from 0.09 to 0.95, and the mean was 0.73; and the genetic distance detected by the AFLP markers ranged from 0.01 to 0.79 with an average of 0.42. All the tested peanut SSR primer pairs were multilocus ones, and the amplified fragments per SSR marker in each peanut genome ranged from 2 to 15 with the mean of 4.77. The peanut cultivars were closely related to each other, and shared a large numbers of SSR and AFLP fragments. In contrast, the species in the genus Arachis shared few fragments. The results indicated that the cultivated peanut （A. hypogaea L.） varieties could be partitioned into two main groups and four subgroups at the molecular level, and that A. duranensis is one of the wild ancestors of A. hypogaea. The lowest genetic variation was detected between A. cardenasii and A. batizocoi, and the highest was detected between A. pintoi and the species in the section Arachis. The relationships among the botanical varieties in the cultivated peanut （A. hypogaea L.） and among wild species accessions in section Arachis and those in other sections in the genus Arachis were discussed.     

《河北农业大学学报》创刊年代考

清光绪二十八年(1902)河北农业大学前身—直隶农务学堂诞生,经几易其名,于1958年更名为河北农业大学至今。清光绪三十一年(1905)直隶高等农业学堂时期创办了《北直农话报》,清光绪三十四年(1908)更名为《直隶农务官报》,中华民国七年(1918)改出《农学月刊》,中华民国十七年(1928)易名为《河大农刊》,中华民国二十三年(1934)更名为《河北通俗农刊》,中华民国二十四年(1935)易名为《河北农林学刊》,1948年更名为《河北农学院研究专刊》,1959年更名为《河北农业大学学报》至今。《河北农业大学学报》前身诸刊都与现时的《河北农业大学学报》有着一脉相承的历史渊源,各刊之间联系紧密,连续性、继承性强。因此,《河北农业大学学报》的创刊时间应追溯至1905年创办的《北直农话报》。     

生态旅游潜在客源市场特征的调查研究--以湖南永州金洞森林旅游开发为例

为探明客源市场生态旅游消费的潜在特征,采用问卷调查的形式,就长沙市居民对湖南金洞生态旅游开发的意向等问题进行抽样调查．结果显示,生态旅游符合人们“回归自然”的旅游新时尚,有着极大的开发空间,指出生态旅游的开发要注重环境保护和可持续发展．开发的产品要以休闲度假类的大众产品为主,开发生态旅游都市客源市场还要多种渠道并用,尤其是要注重媒体的宣传．     

浅谈饲料中有效能的测定技术

饲料中有效能是供动物生长发育的基础.不同动物所用的有效能体系不同,目前大多数动物采用消化能、代谢能体系,但随着研究的发展与深入,发现最能反映饲料有效能的是净能体系.无论哪种体系,采用合理的测定技术准确测定饲料中的有效能值显得尤其重要,通过对饲料有效能值的准确测定可以实现动物所需能量的精确供给,减少养殖成本,使经济效益最大化.文章综述了几种有效能评价体系的测定技术.     

水牛梭形住肉孢子虫包囊抗原的纯化技术

应用萄聚糖凝胶柱层析对水牛梭形住肉孢子虫包囊包溶性抗原进行了纯化。结果表明：纯化水牛梭形住肉孢子虫包囊抗原的最适条件为：选用萄聚糖凝胶Ｇ—１００柱层析系统；洗脱液为０３ＭＰＢＳ（ｐＨ７２），床体积为１０ｃｍ×１６５ｃｍ，上样体积为５００ＨＬ；流速为１２ｍＬ／ｈ。纯化抗原可使琼脂凝胶双扩散试验的阳性检出率提高３０％。     

黑豆不同部分馏油的体外抗氧化性比较

[目的]通过体外抗氧化体系比较黑豆不同部分馏油抗氧化性活性。[方法]通过正交试验优化索氏提取黑豆馏油的最佳工艺,提取黑豆不同部分馏油;研究黑豆不同部分馏油对羟基自由基(·OH)、DPPH自由基(DPPH·)的清除能力。[结果]在样品浓度为1.0 mg/mL时,黑豆不同部分馏油对·OH的清除率分别为全豆馏油83.9%、豆黄(黑豆去皮部分)馏油64.8%、豆皮馏油17.3%,对DPPH·的清除率分别为全豆馏油41.3%、豆黄馏油33.2%、豆皮馏油77.9%。[结论]黑豆不同部分馏油均具有较好的抗氧化性,是良好的天然抗氧化剂。黑豆不同部分馏油对·OH的清除能力从大到小依次为全豆馏油、豆黄馏油、豆皮馏油,对DPPH·的清除能力从大到小依次为豆皮馏油、全豆馏油、豆黄馏油。     

高校贫困生认定工作面面观

国家贫困生资助政策实施以来,对贫困生帮助很大,同时在实际运行中还存在着一些问题。本文提出贫困生认定工作仍需要进一步采取各种相关配套措施,以推动和保障贫困生资助工作更好地开展。     

山茱萸多糖提取工艺优化及马钱苷含量测定

采用L（934）正交设计试验,对山茱萸浸提液中山茱萸多糖的酶水解法提取工艺进行了优化研究,并对浸提液的中有效成分马钱苷含量进行了HPLC法分析。结果表明,山茱萸多糖浸提的最佳工艺为：液料比1∶5,浸提时间4 h,浸提温度80℃,果胶酶添加量0.55 g/L。用HPLC法测定出的山茱萸浸提液中马钱苷平均含量为0.512 ...     

探究板栗的科学贮藏方法

板栗属壳斗科栗属(Castanea mollisima Blume),其种子属于顽拗型种子,不耐贮藏。基于近年来板栗贮藏保鲜技术研究成果,从合理采收、贮前处理、贮藏方法等方面进行论述。     

厚胶合板弹性模量预测模型

为了预测厚胶合板弹性模量,通过简化层合板理论,该文建立了胶合板弹性模量预测模型,并以单板条、经过涂胶热压处理的单板条和相同工艺条件下的单板层积材的弹性模量,采用4种不同铺层方式的19层桉树胶合板对模型进行了验证。结果表明:3种预测值与实测值的趋势一致,相关系数R2顺纹在0.86以上,横纹在0.88以上,但是精度不同。采用单板条弹性模量预测的胶合板弹性模量比实测值偏低;采用经过涂胶热压处理后的单板条弹性模量预测的胶合板弹性模量比实测值偏高;采用相同工艺条件下的单板层积材弹性模量预测的胶合板弹性模量与实测值偏差较小,顺纹平均误差为4.64%,横纹平均误差10.94%。因此,采用相同工艺条件下的单板层积材的弹性模量来预测胶合板的弹性模量是可行的。      

增强我国水果业出口竞争力的思考

分析了入世4年来,我国水果出口在量上实现了突破,但并没有实现质变的主要原因,指出我国水果业存在的问题。论述了引进外资对发展我国水果业的意义,并提出了具体可行的对策与建议。