It is very crucial to evaluate the genetic diversity of peanut genetic resources for identification of peanut germplasm accessions and variety improvement. Cultivated peanut generally has two subspecies, hypogaea and fastigiata. In this study, we identified peanut into three plant types, virginia (var. hypogaea), spanish (var. vulgaris), and valencia (var. fastigiata). Former one belongs to ssp. hypogaea and latter two are involved in ssp. fastigiata. Twenty SSR markers were used to assess the genetic variation of three sets, hypogaea, vulgaris, and fastigiata, respectively. Out of variety-specific SSR primers tried in this study, ten pairs of SSR primers showed polymorphisms. Each accession could be identified by a specific set of polymorphic SSR primers, and allele number was evaluated among accessions, with an average of 6.7 in var. hypogaea and 5.4 in var. vulgaris and fastigiata. For evaluation of genetic diversity, gene diversity ranged from 0.336 to 0.844 and PIC (polymorphism information contents) ranged from 0.324 to 0.827 were investigated. Dendrograms based on genetic distances were constructed, which showed the existence of three different clusters. And these three different clusters might be associated with the genes involved in three plant types. The results also suggested that there were plentiful SSR polymorphisms among peanut germplasm accessions in RDA (Rural Development Administration, Korea) Genebank and SSRs might play an important role in evaluating peanut accessions and cultivar improvement.

The genetic diversity and the genetic relationship among 30 genetic resources of T. officinale and T. coreanum collected from 20 regions in Korea were evaluated by using ISSR markers. Out of 127 loci detected overall, 122 were identified to be polymorphic with a rate of 96.0% at the 30 individuals. The intraspecific polymorphism between T. officinale and T. coreanum was 92.6% and 88.2%, respectively. The genetic similarity matrix (GSM) revealed a wide range of variablility among the 30 accessions, spanning from 0.179 to 922. According to the clustering analysis, different species T. officinale and T. coreanum, were divided into independent groups and all of the accessions could be classified into 7 categories. Especially, all of the mountain collected accessions belonged to independent groups. The study findings indicate that T. officinale and T. coreanum accessions have a high genetic diversity and accordingly carry a germ-plasm qualifying as good genetic resources for breeding.

벼 흰잎마름병은 세계적으로 벼 재배치에서 가장 문제시되는 병해충의 하나이다. 우리나라의 경우 상습발생지를 중심으로 Xa1과 Xa3 이 저항성 유전자로 활용되었으나, 소수의 저항원이 집중적으로 활용됨으로 인해 최근 이병화가 급속히 진행되고 있다. 특히 최근 Xa1과 Xa3 모두를 침해하는 새로운 균계 K3a가 확인됨에 따라 새로운 저항성 유전자의 동정 및 활용의 중요성이 높아가고 있다. 국내육성 자포니카품종 화성벼와 야생벼 O. minuta 간의 종간교잡을 통해 확립된 수원506호의 흰잎마름병에 대한 유전분석을 실시하였다. 수원506호와 통일계 품종인 밀양23호간의 교잡을 통해 확보한 F2 개체들을 활용하여 흰잎마름균주 HB3011 의 접종에 따른 병반장의 변이와 유전자지도 작성에 사용된 SSR 마커의 유전자형간의 연관성분석을 수행하였다. 수원506호의 흰잎마름병 저항성을 지배하며 우성유전자로 작용하는 주동유전인자가 염색체 4변 하단에서 SSR 마커 RM255 에 의해 표지 되었는데, 해당 염색체영역은 Xa1과 Xa2 및 Xa22 등이 보고되었던 영역과 매우 유사할 것으로 추정되었다.

야생벼은 재배벼의 친환경적성을 강화시킬 수 있는 병해충 저항성 및 불량환경에 견딜 수 있는 유용한 유전자들의 보고로 알려져 왔다. 국내에서 육성된 벼 품종인 '화성'(AA게놈)와 야생벼인 Oryza. minuta(BBCC 게놈; Acc.=101141)간의 교잡을 통하여 종간잡종 후대들이 육성되었다. 불화합성과 초기분리세대의 극심한 불임을 극복하기 위해 배주배양으로 F1 개체를 확보하였으며, '화성'으로의 여교잡을 수 차례 실시하였다. 확립된 계통들에 대

본 연구는 사과 품종의 유전적 다양성을 분석하여 육종의 기초 자료로 활용하기 위하여 최근에 국내에서 육성된 품종 및 도입품종을 포함한 34품종을 대상으로 RAPD와 SSR 분석을 수행하였다. RAPD분석에서 총 37종의 선발된 임의 primer를 분석하여 193개의 다형성 밴드(36.2%)를 얻었으며, 평균 다형성 밴드 수는 5.6개였다. SSR 마커 26종을 이용하여 분석한 결과 총 112개의 대립인자가 확인되었고, 마커 당대립인자 수는 평균 4.3개

국내에서 수집된 인삼 자원 중에서 작물학적 특성이 우수하다고 조사된 54점(6~7년 근)을 대상으로 UPOV 조사 기준에 따라 주요 형태적인 특성들을 조사한 결과 경수는 1~4개 범위로 1개인 것이 42.6%이고, 2개인 것이 38.6%로 경수가 1~2개인 것이 전체 81.2%로 나타났으며, 경수가 5개인 것은 없었다. 장엽수는 3~6엽 범위로 5엽이 55.6%였고 4엽인 것은 25.9%였다. 경색은 자색계열이 전체 81.5%로 자색이 46.3%, 연자

We investigated genetic diversity among and within the populations of cultivated ginseng (Panax ginseng C. A. Meyer ) using SRAP profiles. A total of 24 ginseng plants were sampled from the three populations (two from China, one from Korea). Since all these populations are previously shown closely related to each other assister groups, we used Panax quinquefolium L. and wild ginseng as a reference species, which is not "within the sister group". All individuals from the three populations were screened with a total of 36 primer pairs with 26 primers generated from 328 SRAP bands of DNA gels. The mean gene diversity (HE) was estimated to be 0.057 within populations (range 0.032-0.067), and 0.086 at the species level. The genetic differentiation (Gst=0.31) indicates that genetic variation apportioned 30% among populations and 70% within populations. Generally, the result of this study indicates that ginseng contains high molecular variation in its populations.

The polymorphism and the genetic relationships among 32 genetic resources of genus Nelumbo from Korea, Japan, China, USA, India, Thailand and Gabong were thoroughly investigated and extensively examined using ISSR markers. Out of 103 loci detected overall, 94 were identified to be polymorphic with a rate of 91.2%. The genetic similarity matrix revealed a wide range of variability among the 32 accessions, spanning from 0.227 to 0.833. The study findings indicate that the Nelumbo accessions have a high genetic diversity, and accordingly carry a germplasm qualifying as good genetic resources for cross breeding. According to the clustering analysis, different subspecies, N. nucifera and N. lutea, were divided into independent groups and all of the N. nucifera accessions could be classified into five categories. Compared to RAPD analysis, ISSR method showed a clearer picture of polymorphism among the accessions and exhibited a definite distinction even among the subspecies. In this respect, ISSR analysis is considered to be more effective in differentiating the accessions and subspecies of the genus Nelumbo than RAPD test.

Rice lax panicle (lax) mutant had defect in early inflorescence differentiation and lateral branch formation and exhibitedfewer numbers of rachis branches and spikelets in the panicle. The mutant also had abnormality in floral organ formation. Whereas, the spotted leaf 6 (spl6) mutant produced lesions in absence of pathogen. Analysis with a lax spl6 double mutant indicated both genes are controlled by single recessive factor and linked on chromosome 1 with 7 centiMorgan map distance. The lax gene was fine mapped within the 261.3 kb region between RM7594 and RM5389 that predicted 10 open reading frames (ORF) as candidate for lax gene. Sequencing of the candidates in the lax mutant revealed a substitution of nucleotide T by G corresponding to an amino acid substitution from serine (S) to alanine (A) at the 117th position within the coding region of the candidate ORF bhlh123. The intronless 1080 bp cDNA of LAX gene contains an ORF of 215 amino acids and encoded a basic helix-loop-helix transcription factor. Analysis of a 5.1 kb genomic fragment of the lax gene from homozygous dominant progeny which corresponded to indica cultivar resulted in a long deletion of 24 nucleotides in the upstream of LAX cDNA. (This research was supported by the National Research foundation of Korea, Grant 0070065).

In this study, 29 simple sequence repeat (SSR) markers were used to analyze the genetic diversity and population structure of 125 rice accessions from 40 different origins in Africa, Asia, Europe, South America, and Oceania. A total of 333 alleles were detected, with an average of 11.5 per locus. The mean values of major allele frequency, expected heterozygosity, and polymorphism information content (PIC) for each SSR locus were 0.39, 0.73, and 0.70, respectively. The highest mean PIC was 0.71 for Asia, followed by 0.66 for Africa, 0.59 for South America, 0.53 for Europe, and 0.47 for Oceania. Model-based structure analysis revealed the presence of five subpopulations, which was basically consistent with clustering based on genetic distance. Some accessions were clearly assigned to a single population in which >70% of their inferred ancestry was derived from one of the model-based populations. In addition, 12 accessions (9.6%) were categorized as having admixed ancestry. The results could be used to understanding the genetic structure of rice cultivars from these regions and to support effective breeding programs to broaden the genetic basis of rice varieties.

Cowpea might have been introduced from China to Korea and cultivated for several hundred years but it has never been a staple food crop in Korea. In this study, genetic diversity of 492 Korean cowpea landrace accessions that have passport information was estimated using six SSR markers. The mean of Weir's gene diversity was 0.665 from all accessions investigated in the study. Cowpea gene diversity of six local provinces in Korea was ranged from 0.370 in accessions of Gangwon to 0.680 in Jeonra provinces. Low gene diversity of the cowpea genepool of Gangwon province was probably derived from relatively few introductions. Especially SSR markers VM36 and VM39 seem to be good markers to distinguish the Gangwon accessions from others by occurring at a specific locus with higher than 78% of allele frequency. Except for the Gangwon province with the low genetic diversity, gene diversity of cowpea accessions from other provinces was ranged from 0.600 to 0.680 indicating no big differences among provinces. Distribution pattern of the allele frequencies was similar among the other provinces. This may reveal that Korean farmers might exchange cowpea seeds easily with even their neighbors with geographical barriers. A core collection, 100 landraces, ca. 20% of base collection, was developed at the 70% of a similarity coefficient level using random sampling approaches after stratification of the entire landrace collection based on the phenetic dendrogram. The variability of SSR in the base and core collections of Korean cowpea landrace was compared by calculating Weir's gene diversity. The mean of Weir's gene diversity of the core was 0.707 while that of the base collection was 0.665. The higher diversity index in the core collection indicates that it maintains the initial variability and well represents the base collection. The core collection included one of determinate accession (IT 216155) and two of no branching type accessions (IT 103959 and IT 161024). The core collection could be used to guide more efficient management and utilization of the entire collection. This core collection should be revised periodically as additional accessions are collected and further characterization is conducted.

본 연구는 배 유전자원의 유전적 변이를 DNA 수준에서 비교함으로써 육종의 기초 자료로 활용하기 위하여 유전자원 60점을 대상으로 AFLP 분석을 수행하였다. 총 20종의 AFLP 프라이머 조합을 이용하여 522개의 다형성 밴드를 얻었다. 획득된 다형성 밴드를 이용하여 UPGMA 방식으로 유사도 및 집괴분석을 수행한 결과 유전적 유사도 0.691를 기준으로 4개의 그룹으로 분류되었다. 첫 번째 그룹에는 Pyrus communis에 속하는 품종 및 P.

본 실험은 29개 포도 품종(Vitis spp.)의 효율적 유전학적 유연관계를 분석함으로써 포도품종 육성을 위한 기초자료로 이용하고자 RAPD(Random Amplified Polymorphic DNA) 방법을 이용하여 분석하였다. 총 60개의 프라이머를 이용하여 558개의 다형성 밴드를 얻었다. 획득된 다형성 밴드를 사용하여 UPGMA(unweighted pair-group method arithmetic average) clustering 분석 결과

수박에서 종자크기의 유전분석을 위해 종자크기가 다른 6계통을 양친으로 한 교배집단을 조사하였다. 전체 6계통 중 3계통은 수집 계통으로 giant seed(GS)인 'PI525088' big size(BS)인 'Charleston Gray' 그리고 medium seed(NS)인 'NT'를 사용하였으며, 다른 3계통은 보통 크기와 가장 작은 크기 계통간('NT'× 수식 이미지'TDR') 교잡 및 여교잡으로부터 육성되어 종자크기만 상이한 nea

Randomly Amplified Polymorphic DNA (RAPD) was performed to define the genetic variation and relationships of Artemisia capillaris. Fifteen populations by the distributions and habitat were collected to conduct RAPD analysis. RAPD markers were observed mainly between 300bp and 1600bp. Total 72 scorable markers from 7 primers were applied to generate the genetic matrix, and 69 bands were polymorphic and only 3 bands were monomorphic. The genetic dissimilarity matrix by Nei's genetic distance (1972) and UPGMA phenogram were produced from the data matrix. Populations of Artemisia capillaris were clustered with high genetic affinities and cluster patterns were correlated with distributional patterns. Two big groups were clustered as southern area group and middle area group. The closest OTUs were GW2 and GG1 in middle area group, and GB1 from southern area group was clustered with OTUs in middle area group. RAPD data was useful to define the genetic variations and relationships of A. capillaris.