Correlation of vernalization loci VRN-H1 and VRN-H2 and growth habit in barley germplasm.
Increases in yield and adaptation of cereals rest on life cycle adjustments to environmental constraints explained, in part, by the transition from vegetative to reproductive growth, flowering, and maturity [1, 2]. Optimal fitness of developmental patterns to the environment takes place when the crop utilizes most of inputs from the environment on the one hand and on the other hand escapes from deleterious effects of the adverse environmental conditions (i.e., frost stress and late maturity) ,  leading to superior crop performance and yield potential . Barley is a temperate cereal grown in diverse climatic regions from spring growth habit to winter growth habit . Some barley varieties require prolonged exposure to cold temperatures to initiate flowering, a process referred to as vernalization, whereas others initiate flowering without any obligation for vernalization. Therefore, learning more about genetic variation of loci governing vernalization in barley breeding materials is beneficial for developing new cultivars for target environments.
The concept of vernalization sensitivity in barley is different from that in wheat and the sensitivity to low temperature exposure in barley is not an absolute concept. For a vernalization-sensitive wheat, genotype to induce flowering, the seedlings require exposure to low temperatures (46[degrees]C) for 4-6 weeks . The vernalization-sensitive wheat plant does not flower if the vernalization requirement is not fulfilled, whereas an unvernalized vernalization-sensitive barley genotype may induce flowering in late cropping season which is not efficient economically . A three-locus epistatic model of vernalization sensitivity has been proposed by Takahashi and Yasuda , which then was reduced to two-locus epistatic model on the ground that allelic variations in VRN-H3 locus is limited . According to this model, vernalization response in barley is mainly determined by VRN-H1 locus on chromosome 5H and VRN-H2 locus on chromosome 4H, where genotypes with dominant allele Vrn-H2 on VRN-H2 locus and recessive allele vrn-H1 on VRN-H1 locus require the greatest vernalization requirement.
The candidate gene responsible for the VRN-1 locus in wheat and barley is a MADS-box floral meristem identity gene (HvBM5A). High expression of VRN1 is required for the initiation of reproductive development. In some varieties of barley and wheat, MADS-box gene is expressed at high basal levels without requiring a prolonged exposure to cold temperature. Whereas other varieties require prolonged exposure to cold temperature to induce expression of MADSbox at higher levels of expressions required for transition to reproductive stages [10-13]. Further genetic studies revealed that mutations in the promoter or deletions within the first intron of HvBM5A gene lead to dominant Vrn-H1 spring type alleles (nonvernalization requiring) and are known to be responsible for the high level of expression of HvBM5A and the reductions of vernalization requirements in barley [10,13, 14]. Investigation of a large collection of barley germplasm narrowed down the allelic variations of VRN-H1 locus to nine haplotypes (1A, 1B, 2, 3, 4A, 4B, 5A, 5B, and 5C) within the European germplasm [1, 2] of which haplotypes 1A and 5C are typical winter type alleles. The distinction between winter and spring Vrn-H1 haplotypes is based on the presence or absence of the key regulatory element localized in the first intron of barley, a so-called "critical region" [14, 15]. Further investigation of variation in Vrn-H1 winter haplotypes revealed a 486-bp discriminative deletion found only within the solo long terminal repeat (LTR) of haplotype 5C but not on 1A resulting in amplification of 344 bp and 830 bp products in winter haplotypes 5C and 1A, respectively .
The VRN-H2 locus is a dominant repressor of flowering. Genotypes lack a dominant (functional) copy of VRN2 flower early , The candidate gene proposed for Vrn-2 locus in wheat and barley is a ZCCT zinc finger CCT domain transcription factor , Transgenic and RNA interference studies have shown that the ZCCT gene was responsible for the variation in the vernalization requirement in wheat  Loss-of-function or complete deletion mutation in the coding region of this gene leads to recessive spring type vrn-H2 growth habit alleles. The ZCCT candidate gene cluster in VRN-H2 locus consists of three tightly linked genes, ZCCT-Ha, ZCCT-Hb, and ZCCT-Hc , and more references. Laurie et al.  have mapped VRN-H2 locus on the distal part of as mentioned by long chromosome 4H in barley. VRN-H3, the third vernalization locus in barley, is located on chromosome 1H Takahashi and Yasuda . The candidate gene proposed for this locus is HvFT1 which is homologous to the Arabidopsis FT gene [20,21]. The elevated expression of HvFT1 accelerates flower development . Dominant VrnH3 allele results in elevated expression levels of HvFT1. In genotypes requiring prolonged exposure to low-temperature treatment for flower development dominant Vrn-H3 allele provides a bypass of the vernalization requirement . The expression of VRN-H3 is also mediated by a pathway downstream of VRN-H1 and VRN-H2 and interactions with alleles at VRN-H2 and PPD-H1 loci. When a genotype possesses recessive vrn-H2 or vernalization fulfillment represses dominant Vrn-H2, HvFT1 is induced under long-day conditions and accelerates flower development, though this pathway requires active Ppd-H1 allele [22-24].
The barley germplasms grown in Iran are either developed within the country or they were introduced from the ICARDA barley breeding program. The knowledge of germplasm growth habit is limited to flowering in spring sown nurseries. Neither the allelic composition and distribution of vernalization sensitivity loci have been characterized, nor it is clear as to how such allelic variations contribute to the overall adaptation of the country's barley germplasm through the adjustment of flowering time. In this study, we unravel allelic distribution of vernalization loci in barley. The objective of this investigation is the identification of the allelic combinations of VRN-H1 and VRN-H2 loci deployed in a collection of contemporary cultivars by using allele-specific molecular markers and to enhance our understanding of the underlying factors governing overall adaptation of barley to various geographical regions within the barley breeding program.
2. Materials and Methods
2.1. Plant Materials. A total of 51 barley genotypes including cultivars that either developed locally or introduced from external breeding programs, elite experimental lines, and local landraces collected from Iran were selected. The climatic diversity represents regions with moderate temperatures, areas with terminal heat stress, and regions prone to frost stress. In some regions with either moderate temperature or terminal heat stress, the barley production is also under drought and salinity conditions.
2.2. Growth Habit Phenotyping. The growth habit nursery was planted on a single row of one-meter-long plot for each entry during spring 2012 where the minimum temperature did not fall below. Growth habit phenotypes were scored in three categories of W, F, and S representing genotypes with no tiller flowered on the row, some tillers flowered, and all tillers fully flowered, respectively. Genotypes were scored as spring when all tillers of the entire row flowered, as facultative when only few tillers were flowered, and winter when none of the tillers on the entire row flowered by the end of summer 2012.
2.3. DNA Extraction. Small-scale nucleic acid isolation method suitable for marker-assisted selection procedures was used to extract DNA from young leaves of barley genotypes. Fresh leaf tissue of two-week old barley plants were flash frozen in liquid nitrogen and ground into a fine powder. Extraction was performed in 2 mL sterile tubes where a quarter of each 2 mL tube was filled with frozen leaf powder. Then, 0.9 mL of preheated (up to 65[degrees]C) CTAB buffer (2% (w/v) cetyltrimethylammonium bromide, 200 mM Tris/HCl pH 8.0, 20 mM EDTA pH 8.0, 1.4 M NaCl, and 1% (v/v) freshly added [beta]-mercaptoethanol) was added to each tube. Extraction mixes were incubated for 45 min at 65[degrees]C. Precooled chloroform: isoamyl-alcohol mixture (24:1) (0.9 mL) was then added to the heated tubes. The extraction mixes were then centrifuged at max speed (13600 xg) for 15 minutes at 4[degrees]C. The upper layer was then transferred into a new tube and supplemented with 0.7 volumes of precooled (-20[degrees]C) isopropanol and 0.1 volumes of 3 M ammonium acetate. DNA was allowed to precipitate at -20[degrees] C for 45 minutes. The precipitates were pelleted by centrifugation at max speed for 10 minutes at 4[degrees]C. The pellets were washed at least once with 300 [micro]L of precooled 70% (v/v) ethanol. DNA was finally dissolved in 70 [micro]L of nuclease free water.
2.4. DNA Amplifications and Visualization. Deletion-specific primers HvBM5.84F and HvBM5.85R  were used to discriminate between recessive and dominant alleles at VRN-H1 locus based on the presence or absence of the regulatory element in intron I of HvBM5. Thermal cycling profile for these primers consisted of an initial denaturing step of 94[degrees]C for 3 min, followed by 35 cycles of denaturation at 94[degrees]C for 35 s, annealing at 58[degrees]C for 45 s, and extension at 72[degrees]C for 45 s. The PCR reaction was terminated by a final extension of 72[degrees] C for 10 min. The discrimination between two winter haplotypes was assessed by using primers HvBM5A-intronI-F3b and HvBM5A-intronI-R3b after Cockram et al., . PCR was initiated at 95[degrees]C for 3 min, followed by 35 cycles of denaturation at 94[degrees]C for 1min, annealing at 54[degrees]C for 45 s, and extension at 72[degrees]C for 80 s. The PCR reaction was terminated by a final extension of 72[degrees]C for 5 min. Three deletion-specific primer pairs were used to assess the deletions in three-gene cluster VRN-H2 locus that is, ZCCT-Ha, ZCCT-Hb, and ZCCT-Hc [20, 25]. The amplification of a physically linked locus HvSNF2 was also used as a positive control as described by Karsai et al., 2005. Thermal cycling profile for these primers consisted of an initial denaturing step of 94[degrees]C for 4 min, followed by 35 cycles of denaturation at 94[degrees]C for 45 s, annealing at 54[degrees]C for 45 s, and extension at 72[degrees]C for 1 min. The PCR reaction was terminated by a final extension of 72[degrees]C for 10 min. Full list of primer names and sequences are listed in Table 1. PCR reactions of 25 [micro]L contained 1 [micro]L DNA, 2.5 [micro]L 10X Taq buffer, 1.5 mM Mg[Cl.sub.2], 1 [micro]L dNTP mix (2.5 mM of each dNTP), 0.4pmol of each primer, and 1 unit of Taq polymerase. PCR reactions were performed in an Eppendorf Mastercycler (Eppendorf AG, Hamburg, Germany) or T100 Cycler (BioRad Laboratories, Inc., USA). DNA amplifications were visualized, after ethidium bromide staining and separation on 1% or 1.5% agarose gel electrophoresis by using UVItec Gel Document system (UVItec Limited, Cambridge, UK).
3. Results and Discussion
We used allele-specific primers to identify allelic variations of vernalization loci VRN-H1 and VRN-H2 in barley germplasm. We have also evaluated flowering potentials of the germplasm in the spring-sown nursery to establish whether or not they require vernalization for flowering. Three cultivars were used as positive controls in this study. They included cultivars "Nure" and "Igri" with genotype vrnH1/Vrn-H2 (V1w/V2w) as typical winter growth habit and cultivar "Morex" with genotype Vrn-H1/vrn-H2 (V1s/V2w) as a typical spring growth habit . Table 2 represents the relationship between the allelic combinations of VRN-H1 and VRN-H2 and the predicted growth habit. A simplified notation for spring type versus winter type alleles is also provided to avoid confusion of alleles. PCR amplification using primers HvBM5.84F and HvBM5.85R resulted in PCR products of 437 bp in 21 entries with the same size as observed for Nure and Igri, indicating the presence of the vernalization critical region in intron I region of VRN-H1 locus suggestive of winter type recessive vrn-H1 allele (Table 3). Further assessment of these genotypes by means of primer pairs HvBM5A-intronI-F3b and HvBM5A-intronI-R3b resulted in PCR products of 830 bp and 344 bp indicative of winter haplotypes 1A and 5C, respectively (Table 2). Representative gel pictures showing amplifications of 437 bp (vernalization critical region) and discrimination of winter haplotypes 1A versus 5C are shown in Figure 1, respectively. Other genotypes (n = 30) did not yield any PCR products when amplified by primers HvBM5.84F and HvBM5.85R suggestive of a deletion in Vrn-H1 leading to a spring type dominant Vrn-H1 allele (Table 3).
PCR amplification using primers HvSNF2.01F and HvSNF2.04R as positive control primers for Vrn-H2 locus resulted in amplification of a PCR band sized 500-700 bp in all genotypes invariably. When assessed by three ZCCT allele-specific primer pairs, only the positive control "Morex" lacked all three ZCCT genes. Most of the genotypes were characterized as winter type dominant Vrn-H2 allele because they yielded the PCR products of coding regions of ZCCT-Ha (600 bp), ZCCT-Hb (600bp), and ZCCT-Hc (200bp) (Figure 2). In five genotypes, that is, 1-BC-80318, 1-BC-80021, Tokak, ND-82-10, and Nimrooz, the gene ZCCT-Hb was found deleted. Four of the genotypes were characterized by a spring type dominant Vrn-H1 allele and only 1-BC-80318 possessed the full length winter type recessive vrn-H1 allele. In genotype Bereke. (54) both ZCCT-Ha and ZCCT-Hb were absent, and it showed a spring type dominant Vrn-H1 allele (Table 3). Based on a single variety "Fan" observation, Dubcovsky et al.  provided preliminary evidence that, of the three tightly linked ZCCT genes in barley, ZCCT-Hb is not sufficiently deterministic for winter growth habit. One year later, when examining the effect of daylength on expression of VRN-H1 and VRN-H2, Trevaskis et al.  discovered that in a vernalization requiring winter barley the expression of VRN-H1 is not regulated by daylength. In contrast, daylength was shown to reduce the expression of ZCCT-Ha and ZCCT-Hb but not ZCCT-Hc. This may indicate that both ZCCT-Ha and ZCCT-Hb may be sufficiently deterministic for winter growth habit, and deletion of either of the genes may result in the reduced vernalization requirement. Therefore, for the representation of our results, we have decided to denote recessive vrn-H2 where ZCCT-Hb was absent on the basis of the fact that this may reduce deterministic effect of Vrn-H2 locus for a vernalization requirement (Table 3).
In total, 20 genotypes were identified as vrn-H1/Vrn-H2 (V1w/V2w)--a typical genotype for winter growth habit. Almost all entries in this group revealed winter growth habit phenotype in our growth habit nursery except for 1-BC-80392, 1-BC-80207, and 1-BC-80392 that showed facultative growth habit indicating reduced vernalization requirements as compared with others in this group. In this group, a majority of cultivars grouped with landmarks of winter barley genotypes in our study, that is, "Nure" and "Igri" where the VRN-H1 locus harbored the winter haplotype 1A. Cultivars "Bahman," "Goharjo," and "Makoee" are well-adapted winter barley varieties grown in zone C with acceptable levels of winter survival. In contrast, cultivars Karoon and landrace accessions Arigashar and Ashar from Baluchestan Province revealed genotype of vrn-H1/Vrn-H2 (V1w/V2w) where the VRN-H1 locus harbored the winter haplotype 5C.
A total of 24 genotypes were identified as Vrn-H1/Vrn-H2 (V1s/V2w) with expected spring growth habit. These genotypes were grouped with landmarks of spring growth habit barley cultivars in our study, that is, "Yousof" and "Kavir." This group is characterized with a deletion of the vernalization critical region from VRN-H1 intron I. However, in this study we do not report the length of deletion on spring type dominant Vrn-H1 alleles. Therefore, some of these genotypes might represent minimal or reduced vernalization requirements. Various studies have reported that sole deletion observed in the vernalization critical region in VRN-H1 locus may not be sufficient for the removal of the vernalization requirement. Rather, the length of intron I associated with the deletion is more relevant to the reduction in vernalization requirements [27, 28]. Our phenotyping growth habit data revealed that only half of these entries fully flowered in growth habit nursery, and others showed degrees of facultative growth habit. We concluded that there may be variation in length of deletion in VRN-H1 locus amongst genotypes in our study, and therefore, some of these genotypes represent reduced vernalization requirements.
Four germplasms showed vernalization insensitive phenotype due to the lack of a functional ZCCT-Ha and/or ZCCT-Hb alleles in VRN-H2 and the deletion in the vernalization critical region of VRN-H1. These germplasms were Nimrooz, ND-82-10, Tokak, and Bereke-54 which together with Morex revealed complete spring type growth habit. The only entry with the reduced vernalization requirement solely due to the deletion in functional ZCCT-Hb allele in VRN-H2 locus and not due to the deletion of the vernalization critical region was "1-BC-80318". This entry revealed a facultative phenotype in the growth habit nursery.
The barley breeding program in Iran operates on the basis of viewing the country as four mutually distinct climatic characteristics (Figure 3) on the basis of variation in temperature and humidity. This environmental classification has been in place for nearly three decades and includes W-N, W-S, M, and C. The region W-S, characterized by warm and humid climate particularly in reproductive growth stages, is mostly distributed in the north of the country. The regions classified as W-S are mainly in southern Iran and encompass regions with rapidly increasing temperatures in the spring followed by a very hot summer leading to a combined heat and likely drought stress. In region M, the growing season is normally not associated with an extreme temperature or humidity conditions. This region is mostly distributed in the central, western, eastern, and northeastern parts of the country. Regions in zone C are prone to frost damage during the vegetative stage (C), and therefore, winter survival plays a vital role in crop yield.
In Iran, barley is predominantly sown in autumn each year and harvested in the summer of the following year. Spring-sown barley production is not practiced in Iran. What is neglected from this mutual classification of regions--with respect to vernalization requirements--is that nearly all cultivated regions of the country including W-N, W-S, and M are entailed to a mild winter which yet is sufficient for fulfilling vernalization requirements. That explains why some of the cultivars developed or introduced for regions W (Karoon and Jonoob) and M (Nosrat and Rihane) are entailed with full or reduced vernalization requirement. This study drew a baseline understanding of the relationship between genotypes at vernalization loci in barley and growth habit, expected flowering time, and winter survival as related to various geographical regions in an applied barley breeding ground. Genotypic analysis of barley germplasm as represented here increased our awareness of allelic variations in vernalization loci and the adaptation of barley germplasm to various regions of the country. Such information maybe used in breeding practices for designing crosses for recombining allelic forms of VRN in barley and attempting marker-assisted selection for earliness and winter survival. However, further investigation is required to advance our knowledge about SNP variation and InDel evens in VRN-H3 locus and allelic variation in barley photoperiod response loci, that is, PPD-H1 and PPD-H2.
This study was conducted at the Cereals Research Department. The authors are thankful for the Seed and Plant Improvement Institute (SPII) financial support through Grant No. 02-03-03-9012 made available to M. Mohammadi. Special thanks are due to Mr. Ahmad Yousefi, senior barley breeder at SPII.
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Mohsen Mohammadi, Davoud Torkamaneh, and Hamid-Reza Nikkhah
Cereals Research Department, Seed and Plant Improvement Institute (SPII), P.O. Box 4119, Karaj, Iran
Correspondence should be addressed to Mohsen Mohammadi; firstname.lastname@example.org
Received 25 December 2012; Revised 28 January 2013; Accepted 25 February 2013
Academic Editor: Peter Langridge
Table 1: The list of primers names, sequences, and expected PCR product bands used in this study with the original names obtained in the references cited. Vrn-H1 HvBM5.84F 5'-TGAGGGTATGAGTGGCGCTAG-3' 437 bp [+ or -] HvBM5.85R 5'-TCTCATAGGTTCTAGACAAAGCATAG-3' HvBM5A-intronI-F3b 5'-CTTGCATGTGTTGTCGGTCT-3' 344/830 bp HvBM5A-intronI-R3b 5'-GCTGGGACAAGACTCTACGG-3' Vrn-H2 ZCCTH. 14F: 5'-CAAGGAATATCAAGTACATATCTGC-3' 600 bp [+ or -] ZCCTH. 19R: 5'-CCGTATTTATTGAGTTGGTGGTG-3' ZCCTb. 8F: 5'-GCATCAATGCACCCTACCTCTT-3' 600 bp [+ or -] ZCCTb. 11R: 5'-GGAAAACAATGGTGAGAGTAGTACAG-3' ZCCT HcF: 5'-CACCATCGCATGATGCAC-3' 200 bp [+ or -] ZCCT HcR: 5'-TCATATGGCGAAGCTGGAG-3' HvSNF2.01F 5'-CCTGAAGCGAGTATCCATATGC-3' 500-700 bp HvSNF2.04R 5'-GCTGCATTATAGAGAAACAACAACG-3' Vrn-H1 HvBM5.84F Koti et al., 2006  HvBM5.85R HvBM5A-intronI-F3b Cockram et al., 2009  HvBM5A-intronI-R3b Vrn-H2 ZCCTH. 14F: Szucs et al., 2007  ZCCTH. 19R: ZCCTb. 8F: Szucs et al., 2007  ZCCTb. 11R: ZCCT HcF: Yan et al., 2006  ZCCT HcR: HvSNF2.01F von Zitzewitz et al., 2005  HvSNF2.04R Table 2: The predicted growth habit for each genotypic class is listed based on allelic combinations of two-locus VRN-H1/VRN-H2 flowering model. A simplified notation for allelic combinations in relation to growth habit is also provided. Allelic combinations Simplified notation Predicted growth habit vrn-H1/Vrn-H2 V1w/V2w Winter vrn-H1/vrn-H2 V1w/V2s Facultative Vrn-H1/Vrn-H2 V1s/V2w Spring Vrn-H1/vrn-H2 V1s/V2s Spring Table 3: Germplasm evaluated for allelic variations of VRN-H1 and VRN-H2 loci along with their primary cultivation area predicted and observed growth habits are presented. C, M, W-S, and W-N represent cold, moderate, warm-south, and warm-north cultivation regions, respectively. W, F, and S represent winter, facultative, and spring growth habit, respectively. Genotype/germplasm Row Pedigree Regions type cultivated vrn-H1/Vrn-H2 (V1w/V2w) Goharjo 6 Landrace C Michailo Michailo Radical 6 Radical C (CB, ICARDA) Makoee 6 Star/FAO C WA 2196-68/NY6005-18, Bahman 6 F1//Scotia I C Probestdwarf Dasht 2 (France) W L1242 6 L1242 M, C Karoon 6 Strain205 W-S Nure 2 Fior 40/Alpha2//Baraka C Igri 2 820/1427//Ingrid C 1-BC-80392 6 Landrace M, C 1-BC-80453 6 Landrace M, C 1-BC-80458 6 Landrace M, C 1-BC-80395 6 Landrace M, C Shahr-e-kord 6 Landrace Arigashar 6 Landrace W Ashar 6 Landrace W 1-BC-80087 6 Landrace M, C 1-BC-80207 6 Landrace M, C 1-BC-80017 6 Landrace M, C A31vrn-H1/vrn-H2 (V1w/V2s) 1-BC-80318 6 Landrace M, C Vrn-H1/Vrn-H2 (V1s/V2w) MB-87-10 6 82S:510/3/Arinar/Aths//DS 29 M Nosrat 6 Karoon/Kavir M Rihane 6 Rihane M MBS-87-12 6 Roho/Mazorka//Trompilo M Valfajr 6 CI-108985/Egypt M, C Torkaman 6 Rihane04/FAO W-N Gorgan4 2 Herta/Sweden W-N Jonob 6 Gloria "s"/ W-S Copal "s" /CIMMYT Aras 2 Arumir/Europe W-N L.527/Chn-01//Gostoe/4 Yosef 6 /Rhn-08/3/Deir Allal06// M, W DL71/Strain205 20269 6 Kavir/Badia M 20371 6 Legia C, M 1-BC-80162 6 Landrace M 1-BC-80628 6 Landrace M Nik 6 Lignee 527/NK1272//JLB M 70-63 MB-83-14 MB-82-12 2 Novosadski-444 M CIRU/3/AGAVE/SUM EHD-85-8 6 BARD400//MARCO/4/ M PETUNIA 1 Kavir 6 Arivat (Atlas/Vaughn) M Fajr30 6 LigneelSl/Gerbel//Alger- M Ceres/3/Jonoob Teser.93 Teser.93 Sararood 2 Landrace M Badia (20261) 6 Badia M EH-83-7 6 Congona/Borr M MBS-82-5 Salt tolerant (5 shoori) M Vrn-H1/vrn-H2 (V1s/V2s) Tokak 2 Tokak Bereke.54 cold tolerant C Bereke.54 6 adapted to southern Kazakstan C ND-82-10 6 DIO M 1-BC-80021 6 Landrace M Nimrooz 2 Trompillo CMB W-S 74A-432-25B-1Y-1B-1Y-OB Morex 6 Cree/Bonanza M Genotype/germplasm VRN-H1 5C versus HvSNF VRN-H2 VRN-H2 (437 bp) 1A ZCCT-Ha ZCC-Hb vrn-H1/Vrn-H2 (V1w/V2w) Goharjo + 830 (1A) + + + Michailo + 830 (1A) + + + Radical + 830 (1A) + + + Makoee + 830 (1A) + + + Bahman + 830 (1A) + + + Dasht + 830 (1A) + + + L1242 + 830 (1A) + + + Karoon + 344 (5C) + + + Nure + 830 (1A) + + + Igri + 830 (1A) + + + 1-BC-80392 + 830 (1A) + + + 1-BC-80453 + 830 (1A) + + + 1-BC-80458 + 830 (1A) + + + 1-BC-80395 + 344 (5C) + + + Shahr-e-kord + 344 (5C) + + + Arigashar + 344 (5C) + + + Ashar + 344 (5C) + + + 1-BC-80087 + 344 (5C) + + + 1-BC-80207 + 344 (5C) + + + 1-BC-80017 + 344 (5C) + + + vrn-H1/vrn-H2 (V1w/V2s) 1-BC-80318 + 344 (5C) + + - Vrn-H1/Vrn-H2 (V1s/V2w) MB-87-10 - NA + + + Nosrat - NA + + + Rihane - NA + + + MBS-87-12 - NA + + + Valfajr - NA + + + Torkaman - NA + + + Gorgan4 - NA + + + Jonob - NA + + + Aras - NA + + + Yosef - NA + + + 20269 - NA + + + 20371 - NA + + + 1-BC-80162 - NA + + + 1-BC-80628 - NA + + + Nik NA + + + MB-82-12 - NA + + + EHD-85-8 - NA + + + Kavir - NA + + + Fajr30 - NA + + + Teser.93 - NA + + + Sararood - NA + + + Badia (20261) - NA + + + EH-83-7 - NA + + + MBS-82-5 - NA + + + Vrn-H1/vrn-H2 (V1s/V2s) Tokak - NA + + - Bereke.54 - NA + - - ND-82-10 - NA + + - 1-BC-80021 - NA + + - Nimrooz - NA + + - Morex - NA + - - Genotype/germplasm VRN-H2 Predicted Observed ZCCT-Hc GH GH vrn-H1/Vrn-H2 (V1w/V2w) Goharjo + W W Michailo + W W Radical + W W Makoee + W W Bahman + W W Dasht + W W L1242 + W W Karoon + W W Nure + W W Igri + W W 1-BC-80392 + W F 1-BC-80453 + W W 1-BC-80458 + W W 1-BC-80395 + W W Shahr-e-kord + W W Arigashar + W W Ashar + W W 1-BC-80087 + W W 1-BC-80207 + W F 1-BC-80017 + W F vrn-H1/vrn-H2 (V1w/V2s) 1-BC-80318 + F F Vrn-H1/Vrn-H2 (V1s/V2w) MB-87-10 + S S Nosrat + S F Rihane + S F MBS-87-12 + S F Valfajr + S F Torkaman + S F Gorgan4 + S S Jonob + S F Aras + S S Yosef + S S 20269 + S F 20371 + S S 1-BC-80162 + S S 1-BC-80628 + S S Nik + S S MB-82-12 + S F EHD-85-8 + S S Kavir + S S Fajr30 + S F Teser.93 + S S Sararood + S F Badia (20261) + S S EH-83-7 + S S MBS-82-5 + S F Vrn-H1/vrn-H2 (V1s/V2s) Tokak + S S Bereke.54 + S S ND-82-10 + S S 1-BC-80021 + S F Nimrooz + S S Morex - S S
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|Title Annotation:||Research Article|
|Author:||Mohammadi, Mohsen; Torkamaneh, Davoud; Nikkhah, Hamid-Reza|
|Publication:||International Journal of Plant Genomics|
|Date:||Jan 1, 2013|
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