Abstract
Key message
Elite wheat pollinators are critical for successful hybrid breeding. We identified Rht-B1 and Ppd-D1 loci affecting multiple pollinator traits and therefore represent major targets for improving hybrid seed production.
Abstract
Hybrid breeding has a great potential to significantly boost wheat yields. Ideal male pollinators would be taller in stature, contain many spikelets well-spaced along the spike and exhibit high extrusion of large anthers. Most importantly, flowering time would match with that of the female parent. Available genetic resources for developing an elite wheat pollinator are limited, and the genetic basis for many of these traits is largely unknown. Here, we report on the genetic analysis of pollinator traits using biparental mapping populations. We identified two anther extrusion QTLs of medium effect, one on chromosome 1BL and the other on 4BS coinciding with the semi-dwarfing Rht-B1 locus. The effect of Rht-B1 alleles on anther extrusion is genotype dependent, while tall plant Rht-B1a allele is consistently associated with large anthers. Multiple QTLs were identified at the Ppd-D1 locus for anther length, spikelet number and spike length, with the photoperiod-sensitive Ppd-D1b allele associated with favourable pollinator traits in the populations studied. We also demonstrated that homeoloci, Rht-D1 and Ppd-B1, influence anther length among other traits. These results suggest that combinations of Rht-B1 and Ppd-D1 alleles control multiple pollinator traits and should be major targets of hybrid wheat breeding programs.
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Introduction
Bread wheat (Triticum aestivum L.) is an important staple crop for human nutrition and is the third most produced food crop after maize and rice (FAO 2015). To meet rapidly rising world population and future food demands, its production needs to increase. This will require substantial changes in agronomic processes as well as technological advances in crop improvement (Tester and Langridge 2010). Hybrid breeding and the ability to exploit heterosis is one of a few high-priority wheat breeding strategies that has the potential to rapidly improve yield and its stability (Longin et al. 2012; Okada and Whitford 2019; Whitford et al. 2013). In a recent study, yield improvements associated with hybrid vigour were demonstrated to be in the order of 10% increase in grain yield as well as improved resistance against biotic and abiotic stresses (Longin et al. 2013). However, wheat is a highly autogamous plant and has accumulated cleistogamous (closed) flower modifications since domestication. For efficient F1 hybrid wheat seed production, it is important that the male parent is a good pollinator. Ideally, this male parent would be taller than the female parent, exhibit high anther extrusion and have large anthers containing abundant long-life pollen that can be easily dispersed via wind over long distances (Whitford et al. 2013). A large spike containing many well-spaced spikelets would facilitate ease in flower opening as well as pollen dispersal. Most importantly, male pollinators should extrude and dehisce their anthers synchronously with female stigma exertion and receptivity; with pollinators having a prolonged flowering duration (e.g. high tillering). All of these traits, therefore, increase the opportunity for cross-pollination. However, in modern wheat varieties, the genetic resources for elite pollinators are currently limited (Langer et al. 2014; Nguyen et al. 2015).
The genetic basis of several key pollinator traits has been extensively studied, including plant height and flowering time. Semi-dwarfing loci Rht-B1/Rht-D1 were introduced into modern wheats throughout the world resulting in the “Green Revolution” as this trait reduced lodging as well as improving harvest index (Pearce et al. 2011; Peng et al. 1999). The photoperiod sensitivity gene Ppd-1 (Beales et al. 2007; Shaw et al. 2012; Turner et al. 2005) and vernalisation-requirement genes Vrn1 to Vrn4 (Kneipp 2017; Yan et al. 2003, 2004, 2006), each contribute towards controlling flowering time under different environmental conditions. Their influence on plant growth and flowering and how they can be utilised for crop improvements has been extensively studied (Guo et al. 2010; Rebetzke et al. 2007; Wilhelm et al. 2013; Zhang et al. 2008). In addition to plant height and flowering time, anther extrusion (AE) is another pollinator trait that has been extensively studied to unravel the underlying genetic basis. Over the last few years, several studies have revealed that AE is controlled by multiple loci of low to medium effect (Boeven et al. 2016; Buerstmayr and Buerstmayr 2015, 2016; He et al. 2016a, b; Lu et al. 2013; Muqaddasi et al. 2016, 2017a, b; Skinnes et al. 2010; Würschum et al. 2018). Several of these studies showed that Rht-B1/Rht-D1 loci have a medium effect, with the semi-dwarfing alleles (Rht-B1b/Rht-D1b) decreasing AE and increasing anther retention (Boeven et al. 2016; Buerstmayr and Buerstmayr 2016; He et al. 2016b; Muqaddasi et al. 2017b). In contrast, a few other studies using genome-wide association study (GWAS) and a biparental mapping population reported no significant association of Rht-B1/Rht-D1 loci with AE (He et al. 2016a; Muqaddasi et al. 2016, 2017a). This was partly due to a low number of Rht-B1/Rht-D1 lines in the GWAS mapping population (Muqaddasi et al. 2016, 2017a), but it can also be interpreted as Rht-B1/Rht-D1 loci affecting AE only in certain genetic backgrounds. Indeed, Würschum et al. (2018) reported that some of the highest AE pollinator lines carry the semi-dwarfing alleles Rht-B1b or Rht-D1b (Würschum et al. 2018). Thus, genetic association between AE and Rht-B1/Rht-D1 needs further study. Anther length (AL) is also an important pollinator trait and has been shown to have a significant positive correlation with anther extrusion, pollen grain number per anther and pollen mass (Langer et al. 2014; Milohnic and Jost 1970; Nguyen et al. 2015). However, the genetic basis for AL in wheat is limited (Song et al. 2018), especially that contributing to larger size. This holds true for model species such as rice and Arabidopsis, with the exception of reduced anther size often being associated with male sterility (e.g. Binghua and Jingyang 1986; Cheng et al. 2006; Sasakuma et al. 1978). Furthermore, no single genetic locus has been described influencing multiple pollinator traits in wheat, which in turn could play a major role in facilitating cross-pollination for hybrid wheat seed production.
This study aimed at understanding the genetic basis of wheat pollinator traits using both biparental mapping populations and near isogenic lines (NILs). Genetic analysis of two F2 populations identified two AE QTLs, one on chromosome 1B, while the other coincides with the Rht-B1 locus on chromosome 4B. Both loci have a medium effect on AE. The effect of the Rht-B1 locus on AE appears to be genotype dependent and is supported by data derived from several mapping populations and NILs. This study also showed that the Ppd-D1 locus on chromosome 2D is associated with multiple pollinator traits, including AL, spike length (SL), spikelet number (SN) and number of days to heading (DH). Both Rht-B1 and Ppd-D1 loci revealed a significant and consistent effect on AL, which is positively correlated with AE. These results suggest that Rht-B1 and Ppd-D1 are major effect loci and particular allele combinations can be used for selecting a suite of pollinator traits for successful hybrid wheat seed production.
Materials and methods
Plant materials, growth conditions and experimental designs
The bread wheat (T. aestivum L. em Thell) spring-type inbred lines, cid423295sid45 (CIMMYT line: PARUS/3/CHEN/AE.SQ//2*OPATA), Glenwari (GRIS Accession No. K-44557), cid388412sid46 (CIMMYT line: PASTOR//SRMA/TUI/3/SAAR), Gamenya (GRIS Accession No. K-44556) and H1621 (Afghanistan landrace), were selected from spring wheat varieties by pre-screening of AE trait and used to generate F2 mapping populations (Table 1). All experiments were performed in the same glasshouse facility at the University of Adelaide with temperatures ranging from approximately 15 °C (night) to 25 °C (day) and daylight ranging from 12 h (August) to 14.5 h (January). Plants were grown one per pot in 1800 cm3 of coco peat soil, with nine pots placed in a bunding tray. Bunding trays were placed in a two row by five column format (ten trays) on each available bench (Fig. S1). For control and adjustment of measurement data, several plants of each parent of the mapping populations were grown and randomly arrayed across all benches. Mapping populations #1 and #2, which were used for QTL analysis (including ~ 215 F2 plants for each population and ten plants of each parent), were grown between August 2014 and January 2015. Populations #3 and #4, along with additional lines of population #2 (~ 110 F2 plants for each population), were grown between August 2016 and January 2017 to investigate association of Rht-B1 genotype with anther extrusion and other pollinator traits. Most of the near isogenic lines (NILs) were obtained from the Australian Grains Genebank (http://www.seedpartnership.org.au/associates/agg): Rht-B1 in recurrent parent cultivars April Bearded and Mercia carrying Rht-B1a allele (Peng et al. 1999; Youssefian et al. 1992), Rht-D1 in recurrent parent cultivars April Bearded, APD0, Huntsman, Mercia and Nainari carrying Rht-D1a allele (Manske et al. 2002; Peng et al. 1999; Richards 1992; Youssefian et al. 1992), NILs for Ppd-B1 and Ppd-D1 in recurrent parent cultivar Haruhikari carrying Ppd-B1b and Ppd-D1b alleles (Tanio and Kato 2007). Five plants of each NIL and recurrent parent were grown between August 2017 and January 2018 in a randomised design.
Phenotyping and measurement of traits
Generally, six pollinator traits associated with cross-pollination efficiency and two additional traits, partly involved in crossability efficiency, were measured for QTL analysis and marker-trait association studies in F2 mapping populations and NILs. For all traits, the first three spikes of each plant were used for measurements in all experiments and averaged measured value of three spikes was used for QTL analysis. Each spike was tagged at the day of Zadoks scale 57 (Zadoks et al. 1974) with colours used to identify spike emergence order. The following procedures were used to measure the traits: (1) Number of days to heading (DH) were calculated from the date of sowing to the date at Zadoks scale 57 (75% ear emerged from flag leaf), representing flowering time as plants normally initiated flowering 3–4 days after this stage. (2) Visual anther extrusion (AE) was assessed using a scale (0: no AE to 5: high AE) approximately 7 days post anthesis. Each of three spikes was scored independently, according to the flowering time of individual spikes. To ensure consistency and to minimise variation, the same individuals performed all AE trait measurements for all experiments. (3) Anther length (AL) was measured by the following procedure: anthers from primary and secondary florets of two spikelets located at the middle of spike were collected at Zadoks scale 59 (full heading stage) and then stored in a 1.5 mL Eppendorf tube with 70% ethanol at 4 °C. Anther images were subsequently taken using a stereo dissecting microscope Leica MZFL III equipped with the digital camera DFC300 (Leica Microsystems Pty Ltd, Germany). Anther length was then measured directly from the image as a length of polygonal line segments drawn through the centre of the anther. Measurement was performed either manually by using image software FIJI (https://fiji.sc/) (Schindelin et al. 2012) or semi-automatically by using a Matlab (MathWorks, MA, USA) program written for this project (available on request). A minimum of at least five anthers collected for each spike sample was measured. A mean of five anthers from each spike represents AL value of each spike and means of AL values from three spikes were used for further statistical analysis. (4) Plant height (PH) was measured from the soil surface to the base of the flag leaf (mapping populations) or top of spike (NILs) at full maturity. (5) Spike length (SL) was recorded at full maturity and measured from the bottom of the spike to the top of the terminal spikelet excluding awns. (6) Spikelet number (SN) was counted at full maturity. (7) Awnedness (AW) was recorded as the presence or absence of awns. (8) Severe dwarf (SD) phenotype in population #1 was determined by visual assessment of plant stature at 8 weeks. It was also deemed when plant height at maturity was less than 50 cm or the plant contained AA alleles at chromosome 2B locus associated with SD or both. Since the SD phenotype greatly affected all the measured pollinator traits, F2 plants with SD phenotype (51 plants) were excluded from data analysis of population #1 (see details in Supplementary document I).
DNA extraction, marker development and genotyping
DNA was extracted from leaf samples of parental lines and F2 plants as previously described (Rogowsky et al. 1993). Genotyping of populations #1 and #2 was determined by genotyping-by-sequencing (GBS) markers and supplemented by KASP™ markers using a subset of LGC Wheat KASP™ markers (https://www.lgcgroup.com/wheat/#.Wfvz22iCxaQ) and markers for Rht-B1 and Ppd-D1 [CerealsDB: (Wilkinson et al. 2012)] listed in Table S1. Population #3 and #4, additional population #2 and NILs were only genotyped by KASP™ markers for Rht-1 and Ppd-1. KASP™ data were analysed by Kraken™ software (LGC Ltd, UK). GBS libraries for mapping population #1 and #2 were generated as described elsewhere (Elshire et al. 2011; Poland et al. 2012). DNA concentration was quantified by a standard PicoGreen (Thermo Fisher Scientific) assay and 200 ng of genomic DNA was digested by PstI and MspI restriction enzymes at 37 °C for 2 h, followed by ligation with 96 multiplex oligo adapters. Subsequently, all samples in the 96-well plate were pooled into a single 1.5 mL tube and pooled DNA was purified by ISOLATE II PCR and Gel Kit (Bioline, UK). The multiplex libraries were amplified by PCR and sequenced by Illumina HiSeq (Illumina Inc, USA) to obtain 150 bp paired-end sequences, according to the manufacturer’s instruction. Genotypes for each individual were determined from the sequence data using an analysis pipeline as described elsewhere (Watson-Haigh and Eckermann, in preparation). Briefly, reads were aligned to the IWGSC RefSeq v1.0 genome assembly and the position of homozygous and polymorphic SNPs observed in the parent data was used to call SNPs in the F2’s. The GBS markers developed and used for linkage map construction of populations #1 and #2 are listed in Tables S2 and S3.
Linkage map construction, QTL analysis and statistics
Genetic linkage maps for populations #1 and #2 were generated by utilising the R package ASMap (Taylor and Butler 2017). Summary information for the linkage maps is shown in Table S4. Phenotypic data from the experiments in the first year (populations #1 and #2) were spatially analysed using ASReml (Gilmour et al. 2009) which was possible due to the replication of parental lines. For each trait, tray, row and column effects (Fig. S1) were fitted as random effects and lines fitted as fixed effects, which enabled best linear unbiased estimators (BLUEs) to be calculated for each F2 and parental line. QTL analysis was performed using the “scanone”, “makeqtl”, “addqtl”, “refineqtl” and “fitqtl” from the R/QTL package (Broman et al. 2003), using all significant QTLs as covariates. A permutation test (using 1000 permutations) was used to set a LOD score threshold of 3.7 that corresponded to a genome-wide significance level of 0.05. Only QTLs above this threshold have been reported in this study in order to focus on higher effect QTL. Percent of phenotypic variation explained by QTL and the additive effect of the higher allele were also calculated. Summary statistical data for mapping populations, Pearson’s correlation analysis, analysis of variance (ANOVA) for marker-trait association, and graphs (histogram, box plot, jitter plot and scatter plot) were produced by using GenStat ver15 (VSN_International 2011) and RStudio (RStudio_Team 2015).
Locating markers and genes/loci of interest on the Chinese Spring physical map
We mapped the following markers/genes/loci to IWGSC RefSeq v1.0, the Chinese Spring (CS) reference sequence assembly (International Wheat Genome Sequencing 2018); (1) GBS and KASP™ markers used in this study (Tables S1–S3), (2) markers corresponding to the QTL peak of pollinator traits identified in this study, (3) anther extrusion loci and their associated markers reported previously, where sequence information was available (Table S5) and (4) phenology genes/loci associated with flowering time and plant/floral architecture in rice, barley and wheat (Table S6). Marker and gene sequences were used for BLAST searches against the IWGSC RefSeq v1.0 and top hits with a significant similarity (100% identity or e value < 1E − 20) to the expected chromosome, according to the literature, were used for mapping location on the CS physical map. Markers which showed multiple BLAST hits with similar e value to the same chromosome, they were not included in the map. The start sequence position (in Mb) of the BLAST alignment was used, and a physical map for each chromosome was generated using MapChart (Voorrips 2002).
Results
Development of genetic mapping populations and correlations of pollinator traits
Five spring wheat lines were used in this study to develop F2 mapping populations, and they exhibited contrasting phenotype for a range of pollinator traits, especially AE and AL (Table 2). CIMMYT lines cid423295sid45 and cid388412sid46 were used as low AE parents, while Glenwari, H1621 and Gamenya were used as high AE parents. All mapping populations have allelic variation for Rht-B1 and Ppd-D1, while all parental lines were monomorphic for Rht-D1a allele. Over 200 F2 plants of populations #1 (cid423295sid45 × Glenwari) and #2 (cid388412sid46 × H1621) were phenotyped for plant height (PH), days to heading (DH), anther extrusion (AE), anther length (AL), spike length (SL) and spikelet number (SN). We observed a generally normal distribution for all six pollinator traits in population #1 (excluding SD plants; see Supplementary document I) and population #2 (Fig. S2). Since F2 plants were used for phenotyping, we used replicated parental plants in order to adjust F2 measurements for spatial and environmental effects derived from slight differences in growing conditions. Parental lines clearly exhibited large genetic variation for most traits relative to that deemed to be environmental variability based on parental replicates (Fig. S3). This indicated that the populations exhibited a significant genetic variance between F2 individuals. We investigated correlations between pollinator traits, especially anther traits, in order to understand their functional relationship. In population #1, we found a moderate negative correlation between AE and DH and also that AL was moderately and positively correlated with DH, PH, SL and SN (Table 3). In population #2, AE was weakly and positively correlated with AL and PH, whereas a negative correlation between AE and DH was observed to be weakly significant. AL was moderately correlated with SL and weakly with PH and SN. Overall, correlations of AE with other traits are generally weak, while AL correlated relatively higher with other traits in these two populations. These findings indicate that the physiological mechanisms and genetic factors responsible for determining AL may have more commonality with those determining flowering time, stature and floral organ size.
QTL analysis in F2 population #1 identified a major effect of Ppd-D1 locus on multiple pollinator traits
F2 populations #1 and #2 were genotyped by GBS and KASP™ markers using approximately a thousand markers for each population (Tables S1–S3). Genetic linkage analysis resulted in 21 linkage groups for both populations, corresponding to each of the wheat chromosomes, with total genetic map size of over 4000 cM for each population (Table S4). Linkage maps for D chromosome tended to have fewer markers, e.g. 4D and 5D, due to shorter chromosome size and less availability of polymorphism, compared to those of A and B chromosomes. QTL analysis was conducted for all six pollinator traits as well as awnedness (AW) and severe dwarf (SD) in population #1. A strong QTL for AW at the distal end of chromosome 5A (Fig. S4a and Table 4) was identified which was co-located with the well-known dominant B1 locus for awn inhibition (Kosuge et al. 2008). This provides confidence that the approach for linkage map construction and QTL analysis in this paper is able to accurately detect true loci.
QTL analysis in population #1 identified a single AE QTL of medium effect on chromosome 1B with LOD score of 5.88, explaining 15.5% of the phenotypic variation, for which the high allele is derived from elite pollinator parent Glenwari (Fig. 1a and Table 4). Similarly, a single AL QTL of medium effect was identified on chromosome 2D, with Ppd-D1 as the closest marker to the QTL peak and the Glenwari Ppd-D1b photoperiod-sensitive allele having a positive effect (Fig. 1a and Table 4). This Ppd-D1/2D QTL was also significantly associated with DH, SL, SN indicating a major effect on these traits. A single PH QTL with major effect was identified at the Rht-B1 locus on chromosome 4BS, and no other PH QTLs were detected. In this population, we were unable to confirm a genetic association between Rht-B1 and AE trait where the LOD score at the Rht-B1 marker was 0.73. However, in the AL QTL analysis, the LOD score at the Rht-B1 marker was 2.45 which was below the threshold but does indicate some evidence for an effect on AL (see also Fig. S5a). Therefore, in population #1, allelic variation at Rht-B1 does not affect AE, but may have a small effect on AL.
Rht-B1 locus is associated with anther extrusion in F2 population #2
In contrast to population #1, the Rht-B1 locus on chromosome 4B was identified as a major QTL for AE in population #2, with LOD score of 8.83, explaining 15.4% phenotypic variation (Fig. 1b and Table 4). This strong AE QTL was evident despite the 4B linkage map containing fewer markers and missing distal 4BS markers (Fig. 1b). An additional minor AE QTL was found on 6B spanning a broad region (148 cM, 95% confidence interval in Fig. S4b). This indicates a large uncertainty about the location of a QTL in this region, or possibly indicates the presence of multiple minor QTLs. As expected, the Rht-B1/4B locus was identified as a major QTL for PH and this QTL was also associated with SL. It should be noted that the Rht-B1 locus corresponds to the second AL QTL peak on 4B, exhibiting a LOD score of 3.80 (Fig. 1b), while the first AL QTL peak was detected at 40 cM position on 4B. For these pollinator traits AE, AL and PH, the Rht-B1a tall wild-type allele derived from elite pollinator parent H1621 had a positive effect (Fig. S5a).
Similar to population #1, the Ppd-D1/2D locus showed a significant association with multiple traits including DH, SL, SN and AL with medium to high effects (Fig. 1b and Table 4). Again, the Ppd-D1b photoperiod-sensitive allele derived from the elite pollinator parent H1621 had a positive effect on all of these traits. We identified two additional QTLs for DH on 2A and 5B with medium–high effect and these QTLs were co-located with PH QTLs (Figs. 1b, S4b). However, none of these DH/PH QTLs showed associations with either AL or AE. Overall, Rht-B1/4B and Ppd-D1/2D loci have significant effects on multiple pollinator traits, with the tall Rht-B1a and photoperiod-sensitive Ppd-D1b alleles being associated with favourable pollinator traits.
Rht-B1 locus affects anther extrusion in a genotype dependent manner
We observed contrasting results for genetic association between the Rht-B1 locus and trait AE in populations #1 and #2 (Fig. 1 and Table 4). This difference may be caused by allelic variation, not only of the Rht-B1 gene itself but also other genes closely linked to the locus, and/or interaction between parental genetic backgrounds and epistatic interactions. Therefore, we subsequently investigated potential phenotypic variation in Rht-B1 locus containing wild-type tall Rht-B1a allele between elite pollinator parents. We developed two additional F2 populations by crossing the same low AE parent cid388412sid46 as population #2 and two different high AE parents, Gamenya for generating population #3 and Glenwari for population #4 (see “Materials and methods” section and Tables 1, 2).
The Rht-B1 genotype was significantly associated with PH across all three populations (Fig. 2a), although additional dwarfing genes derived from Gamenya appeared to be present in population #3 as it has short stature (Table 2). We again found a significant association between Rht-B1 genotype and AE in population #2, confirming our previous result (Figs. 2b, S5), but found no association in population #3 and only weak association in population #4. Furthermore, the same high AE parent Glenwari was used in population #1 and #4 and revealed slightly different effect of Rht-B1 locus on AE trait for these two populations. These results suggest an epistatic effect on AE between Rht-B1 locus and the genetic background.
This was further investigated by using near isogenic lines (NILs) of the Rht-B1 locus in two different recurrent parent cultivars (April Bearded and Mercia), minimising genetic background effect. Summary statistics for traits in NILs used in this study are shown in Table S7. NILs containing the Rht-B1b dwarf allele showed a significant reduction in PH as expected (Fig. 3). The Rht-B1 locus also showed a significant association with AL in both NILs, which is consistent with AL QTL results for population #2 (Fig. 1). However, we found relatively larger trait variation in AE and no significant association with AE was identified in both NILs. These results further support our observation that an effect of Rht-B1 allele on AE is genotype dependent, whereas there is more consistent association of Rht-B1 locus with AL across genetic materials.
Rht-D1 and Ppd-1 loci influence anther length
We also investigated the effect of Rht-D1 and Ppd-B1 and Ppd-D1 loci on various pollination traits by using NILs. The Rht-D1 NILs in all five recurrent parent backgrounds clearly showed a significant and consistent association with PH and AL (Fig. S6). All NILs containing semi-dwarfing Rht-D1b allele exhibited reduced PH and AL. The association with AE differed among recurrent parent genotypes, with three NILs (APD0, Huntsman and Nainari) showing a significant association with reduced AE, Mercia NIL having no significant association and April Bearded NIL having opposite association with increased AE. In contrast to results for the Rht-B1 NILs, Rht-D1 allelic variation showed no association with SL in three NILs (April Bearded, APD0 and Nainari). Indeed, an opposite effect was observed in two NILs (Huntsman and Mercia), indicating that the Rht-D1b semi-dwarfing allele is associated with longer spikes for these two genetic backgrounds (Figs. 3, S6).
Four types of Ppd NILs in spring wheat photoperiod-sensitive variety Haruhikari background (Tanio and Kato, 2007) were used in this experiment. NILs H(A) and H(B) carry the Ppd-D1a photoperiod-insensitive allele derived from Saitama27 and Fukuwasekomugi, respectively. H(C) NIL contains Ppd-B1a insensitive allele and H(D) carries Ppd-B1a and Ppd-D1a alleles derived from Fukuwasekomugi. As expected for the growing conditions, all NILs flowered significantly earlier than the recurrent parent line (Fig. S7). They also all exhibited significantly reduced AL except for the H(B) NIL. Similarly, both Ppd-D1 and Ppd-B1 NILs revealed a weak association with AE. Furthermore, Ppd-D1 NILs [H(A) and H(B)] showed a strong association with SL. These results further confirmed the association of the Ppd-D1 locus with multiple pollinator traits, especially AL and SL with the photoperiod-sensitive Ppd-D1b allele being associated with favourable pollinator traits (Figs. S5 and S7).
Physical location of anther extrusion loci and phenology genes in Chinese Spring reference genome map
AE or anther retention is reported to be controlled by multiple genetic factors of weak to medium effect in both spring- and winter-type wheat (Boeven et al. 2016; Muqaddasi et al. 2016, 2017a). However, all the reported genetic analyses for AE have been done by using different genetic mapping populations, including double haploid (Buerstmayr and Buerstmayr 2016; He et al. 2016a; Lu et al. 2013), recombinant inbred lines (Buerstmayr and Buerstmayr 2015; He et al. 2016a; Lu et al. 2013), backcross populations (Buerstmayr and Buerstmayr 2016) and association mapping populations (Boeven et al. 2016; Muqaddasi et al. 2016, 2017a; Würschum et al. 2018). It would be most valuable for breeding purposes if we could identify common AE QTLs in these studies. To achieve this, we mapped all the AE loci, including pollinator trait QTLs identified in our study, onto the Chinese Spring (CS) IWGSC RefSeq v1.0 physical map (International Wheat Genome Sequencing 2018). In addition, we mapped wheat phenology genes/loci associated with flowering time and plant/floral architecture to investigate physical distance between AE loci and phenology genes/loci.
GBS and KASP™ markers used in this study were also mapped to get an estimate of differences between genetic distance and physical distance in the CS reference genome. These markers were mapped to a greater extent in the distal chromosomal regions and less frequently in the central region, which indicates that centromeric or repetitive genomic regions act as marker poor domains (Fig. S8). A comparison of marker position and order in the genetic and CS physical maps shows differences between the two maps and where disagreements exist (Figs. 4, S9). The AE QTL we identified on chromosome 1B (qAE_P1.1) appears to be located near three other previously identified AE loci (Fig. 4a). About the broad AE QTL on 6B (qAE_P2.2) identified in population #2, we found one known AE locus mapped relatively close to the QTL peak and several others located within broader QTL region (Fig. S9). Three known AE loci are physically closely located with Ppd-D1 on chromosome 2D (Fig. 4b). There are a few other phenology genes/loci (e.g. Rht8, WFZP and Tg-D1) located nearby, which also could potentially affect the AE trait. Furthermore, there are several loci containing a few AE QTLs identified in common from independent genetic mapping projects, including regions on chromosome 2B near Ppd-B1 and Tg-B1, 4B at Rht-B1, 4D at Rht-D1 and 5B near VRN-B1 (Fig. S8). It is reasonable to find that these AE loci are closely mapped to phenology genes, as such genes tend to have pleiotropic effect. Table S8 summarises physical position of AE loci and phenology genes that are located nearby (also see Fig. S8). These highlight the complexity of AE trait control as a result of contributions by multiple genetic loci and potential association with genes involved in flowering time and plant/floral architecture.
Discussion
Effect of Rht-1 on anther extrusion
The use of elite pollinators is critical for hybrid wheat breeding programs. This requires multiple traits that have rather complex biological and physiological mechanisms and that are controlled by multiple genetic factors. Among these traits, AE is positively correlated with PH (Table 3 and Boeven et al. 2016; Langer et al. 2014; Lu et al. 2013) and associated with semi-dwarfing Rht-1 loci (Boeven et al. 2016; Buerstmayr and Buerstmayr 2016; He et al. 2016b; Lu et al. 2013). In our study, we have shown that the effect of Rht-B1 locus on AE is genotype dependent; only two out of four F2 populations investigated revealed a significant association (Figs. 1, 2 and Table 4). A few previous GWAS studies did not find an association of AE with Rht-B1 locus, partly due to the small number of plants carrying Rht-B1b semi-dwarfing allele in the mapping population (Boeven et al. 2016; Muqaddasi et al. 2016, 2017a, b), and another study showed no significant association of Rht-D1 locus with AE in a population of 131 RILs (He et al. 2016a). Combined with our results, Rht-B1 appears to affect AE in a more genotype dependent manner, whereas Rht-D1b semi-dwarfing allele tended to show a stable negative effect. Nevertheless, high AE wheat accessions carrying semi-dwarfing alleles of Rht-B1b or Rht-D1b do exist (Würschum et al. 2018). Genotype dependency of Rht-1 association with AE may be explained by the requirement of multiple biological processes for this trait. At anthesis, lodicule swelling induces flower opening followed by anther filament elongation and therefore anthers extrude. Shape of spikelet and floret, spikelet spacing, lodicule and anther size, filament length and glume stiffness are all likely to play a role in influencing the level of flower opening and anther extrusion process. Positive correlation between AE and AL (Table 3), AE and AL plus filament length (Langer et al. 2014) and co-localisation of glume stiffness and AE QTLs (He et al. 2016a) partly supports this idea. Some influencing factors listed above may affect AE more positively, overcoming negative effects of Rht-1 semi-dwarfing alleles.
Rht-1 encodes a DELLA protein which plays a part in the gibberellin signalling pathway and is involved in various growth processes such as seed germination, stem elongation, leaf expansion, trichome development, pollen maturation, and the induction of flowering (Daviere and Achard 2016; Pearce et al. 2011). Therefore, mutation of this gene generally causes pleiotropic effects. Our genetic study revealed that Rht-B1 locus is not only associated with AE and PH, but also AL and SL (Figs. 1, 3, S5 and Table 4). We also showed a significant association of Rht-D1 with AL (Fig. S6). Thus, Rht-1 is involved in multiple traits influencing AE process, including spikelet spacing (SL), anther size (AL), glume stiffness (Buerstmayr and Buerstmayr 2016), and filament elongation (Youssefian et al. 1992). This could explain why Rht-1 is the most effective QTLs for AE.
Tall male pollinators with high AE associated with Rht-B1a or Rht-D1a wild-type alleles are desirable for hybrid seed production. However, F1 hybrids would inherit tall alleles, which is likely to be highly undesirable in some environments. Semi-dwarf wheats yield more and are typically selected for hot and dry climates (Alghabari et al. 2014; Kowalski et al. 2016; Tricker et al. 2018). It might be possible to use other Rht genes for introducing semi-dwarf trait. The Rht24 locus, for example, did not show a significant effect on AE (Würschum et al. 2018). We also confirmed that there is no known AE QTLs nearby Rht24 on chromosome 6A (Fig. S8). Therefore, Rht24 could be used to select semi-dwarf wheat plants without affecting AE trait (Würschum et al. 2018). Other Rht loci (Rht12/5A, Rht23/5D, Rht13/7B) did not co-locate with any known AE loci on the CS physical map, providing potential alternative semi-dwarfing genetic resources. In specific genetic backgrounds, it might also be possible to use semi-dwarfing allele Rht-B1b for controlling plant height without compromising AE (Figs. 2, 3). Better understanding of the effect of different Rht genes on AE and other pollinator traits could provide us with a greater choice of dwarf genetic resources to design superior hybrids in breeding programs.
Pleiotropic effect of Ppd-D1 locus on pollinator traits
Optimal co-occurrence of flowering time between the male and female plants is one of the most important key factors in ensuring successful hybrid seed production. We have shown that Ppd-D1 locus not only affects flowering time (DH), but is also associated with important pollinator traits SL, SN and AL (Figs. 1, 4b). Anther size represented by AL is strongly correlated with pollen mass (Milohnic and Jost 1970; Nguyen et al. 2015; Pickett 1993). A long spike containing many well-spaced spikelets would facilitate flower opening as well as pollen dispersal, therefore favourable pollinator traits. Moreover, we found that Ppd-D1 is weakly but significantly associated with AE in population #1 and NILs (Figs. S5b and S7), and three AE QTLs closely located with Ppd-D1 (Fig. 4b) were identified in other studies (Boeven et al. 2016; Muqaddasi et al. 2016, 2017b). Similarly, Ppd-B1 showed a significant association with AE and AL (Fig. S7) and two AE QTLs (Boeven et al. 2016; Muqaddasi et al. 2017a) mapped nearby Ppd-B1 linked markers on chromosome 2B (Fig. S8). These demonstrated a pleiotropic effect of Ppd-1 loci on multiple pollinator traits.
Ppd-1 encodes a pseudo-response regulator involved in the regulation of CONSTANS (CO) gene expression and upregulation of VRN3/TaFT, accelerating flowering under long days in wheat and barley (Distelfeld et al. 2009; Turner et al. 2005). In wheat, the semi-dominant photoperiod-insensitive Ppd-D1a allele has a deletion in the promoter that causes miss-expression of this gene and increased expression of VRN3/TaFT under short days, therefore inducing early flowering (Beales et al. 2007). Investigation of six haplotype variations of Ppd-D1 revealed a significant haplotype effect on various agronomic traits, not only DH but also SL, SN and PH (Guo et al. 2010). It would be interesting to explore the effect of different Ppd-D1 haplotypes on AL and AE traits as we found in H(A) and H(B) NILs (Fig. S7). Another allelic variant of Ppd-D1 caused a change in spike architecture, forming paired spikelets (Boden et al. 2015), which could also influence pollinator ability. Therefore, Ppd-D1 has a major effect on multiple pollinator traits and specific effects of haplotype variants on these traits needs to be investigated further.
Elite pollinators for hybrid wheat breeding
Mapping of known AE loci on wheat genome sequence (Fig. S8) highlighted the presence of multiple genetic factors associated with this trait, with each locus having a relatively minor effect (Muqaddasi et al. 2017a; Würschum et al. 2018). A comparison between our genetic linkage maps and CS physical map revealed a close link between AE QTLs (1B and 6B) and other flowering time genes/loci (Figs. 4a and S9). TaFDL2 (Abe et al. 2005; Li and Dubcovsky 2008) and HvFT3 (Halliwell et al. 2016; Mulki et al. 2018) are closely located to 1B QTL, while several CO genes (Griffiths et al. 2003; Nemoto et al. 2003) and TaTOC1 (Zhao et al. 2016) are located within the broad 6B QTL. These genes are not only involved in flowering time, but many are known to have a pleiotropic effect on floral development; therefore, they may be affecting the AE trait. Nevertheless, these phenology genes, including Rht-1 and Ppd-1, often affect flowering time as well as major agronomic traits (Guo et al. 2010; Richards 1992; Wilhelm et al. 2013; Youssefian et al. 1992). Since these are critical traits not only for hybrid seed production but also for general inbred line breeding, breeders may have limited scope for genotype selection beyond key phenology genes/loci already used in their current breeding program. Identifying new AE QTL loci with a significant effect within wheat genetic resources is one strategy, while the introgression of chromosome segments from related cross-pollinating grass species like rye could be another strategy to manipulate floral structure of wheat (Nguyen et al. 2015).
A more practical approach would rely on genomic selection for pyramiding multiple AE loci and other pollinator traits carrying favourable alleles and for predicting pollinator traits, flowering time and hybrid performance at the same time (Boeven et al. 2016; Okada and Whitford 2019). It is important to note that AE is a critical trait for hybrid seed set (Boeven et al. 2018), but not a sole trait determining elite pollinators. Many spikelets containing large anthers increase the total amount of pollen available for dispersal and these traits are under independent genetic control. Furthermore, female parent traits such as flower opening (Okada et al. 2018), stigma receptivity and length (Pickett 1993) are also critical and the genetic basis of these traits is still largely unknown in wheat. Prioritising pollinator traits in breeding selection programs is essential, and this will be facilitated by quantitative assessment of each pollinator trait and its impact on cross pollination efficiency. With recent advancements in phenotyping platforms (Ghanem et al. 2015; Gils et al. 2013; Jimenez-Berni et al. 2018), and the availability of wheat genomic resources (International Wheat Genome Sequencing 2018) and the implementation of new genetic modelling tools (Miedaner et al. 2017; Zhao et al. 2015), there is a real potential to breed elite pollinator lines, pyramiding multiple favourable traits and achieving superior performance in F1 hybrids at the same time.
Author contribution statement
TO, RJ, UB, MA, PW and RW planned and designed the research. TO, RJ, PE, NW, PW, YH, MB, ET and HL performed experiments. TO, RJ, PE, NW, YH, MB and ET analysed data. TO, RW, RJ, MA, PW, KK, MA, YH, DF and UB discussed results and interpretation of data. TO wrote the manuscript, and TO, PW, NW, PE, UB, RW edited the manuscript. All authors reviewed the manuscript.
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Acknowledgements
This research was supported by DuPont—Pioneer Hi-Bred International. We thank David Correia, Yuriy Onyskiv, Vy Nguyen, Alex Kovalchuk and Dr Ursula Langridge for assisting with glasshouse work. We also thank Drs Radoslaw Suchecki and Beata Sznajder for data analysis and Dr. Ajay Sandhu for critical advice for the project. We also thank Margaret Pallotta for technical advice and critical reading and editing of the manuscript.
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Table S1.
KASPTM markers used for developing genetic linkage map for populations #1 and #2. Table S2. GBS markers used for developing genetic linkage map for population #1. Table S3. GBS markers used for developing genetic linkage map for population #2. Table S4. Summary information for genetic linkage map and QTL analysis for population #1 and #2. Table S5. A list of genetic loci associated with anther extrusion reported in the previous publications. Table S6. Phenology genes mapped on Chinese Spring reference sequence IWGSC RefSeq v1.0 to compare physical location of genetic loci associated with pollinator traits. Table S7. Summary statistics for evaluated traits in Rht-1 and Ppd-1 NILs used in this study. Table S8. Physical location of AE loci and flowering time (FT) or plant/floral architecture (FA) genes/loci in CS reference map IWGSC RefSeq v1.0 (XLSX 483 kb)
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Okada, T., Jayasinghe, J.E.A.R.M., Eckermann, P. et al. Effects of Rht-B1 and Ppd-D1 loci on pollinator traits in wheat. Theor Appl Genet 132, 1965–1979 (2019). https://doi.org/10.1007/s00122-019-03329-w
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DOI: https://doi.org/10.1007/s00122-019-03329-w