Abstract
Chinese cabbage (Brassica rapa L. ssp. pekinensis) is one of the most important vegetables in China. Genetic dissection of leaf mineral accumulation and tolerance to Zn stress is important for the improvement of the nutritional quality of Chinese cabbage by breeding. A mapping population with 183 doubled haploid (DH) lines was used to study the genetics of mineral accumulation and the growth response to Zn. The genetic map was constructed based on 203 AFLPs, 58 SSRs, 22 SRAPs and four ESTPs. The concentration of 11 minerals was determined in leaves for 142 DH lines grown in an open field. In addition shoot dry biomass (SDB) under normal, deficient and excessive Zn nutritional conditions were investigated in hydroponics experiments. Ten QTLs, each explaining 11.1–17.1% of the Na, Mg, P, Al, Fe, Mn, Zn and Sr concentration variance, were identified by multiple-QTL model (MQM) mapping. One common QTL was found affecting SDB under normal, deficient and excessive Zn nutritional conditions. An additional QTL was detected for SDB under Zn excess stress only. These results offer insights into the genetic basis of leaf mineral accumulation and plant growth under Zn stress conditions in Chinese cabbage.
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Introduction
Chinese cabbage (Brassica rapa L. ssp. pekinensis) is one of the most important vegetable crops in China with, among vegetable crops, the largest cultivation area and per capita consumption. It is a main source of mineral nutrients for the Chinese population (Ma et al. 2007), and therefore elevating the amount of beneficial minerals in Chinese cabbage can contribute to the reduction of micronutrient malnutrition in China. The improvement of mineral content by plant breeding, also referred to as biofortification (Bouis 2002), is a recent development that requires knowledge about the genetic variation for this trait and genetic markers linked to relevant genes (reviewed in Ghandilyan et al. 2006). However, genetic studies on mineral content in crops have been limited mainly to seeds, such as for common bean (Beebe et al. 2000; Islam et al. 2002), rice (Gregorio et al. 2000), wheat (Monasterio and Graham 2000), maize (Banziger and Long 2000) and also the model species Arabidopsis thaliana (Vreugdenhil et al. 2004). QTLs were also identified for mineral concentrations in leaves for P (Bentsink et al. 2003), Cs (Payne et al. 2004) and K (Harada and Leigh 2006) in A. thaliana and for Zn in Thlaspi caerulescens (Assunção et al. 2006; Deniau et al. 2006). These studies have demonstrated the presence of allelic variation affecting mineral accumulation, although the identity of the underlying genes remains unknown. However, very little is known about the genetics of mineral concentration in leafy vegetables, such as B. rapa vegetables, until recently QTLs were identified for shoot Ca and Mg concentrations in Brassica oleracea (Broadley et al. 2008).
Zn is an essential micronutrient as it plays both functional and structural roles in enzyme reactions (Vallee and Auld 1990). However, both Zn deficiency and Zn toxicity occur worldwide, including in China, depending on Zn content and availability in the soils (Nan and Zhao 2000; Hacisalihoglu and Kochian 2003; Liu et al. 2005). In addition to reduced yield due to Zn deficiency or toxicity, the transfer of excess Zn from soils to plants is an important contribution to human health exposure to Zn and more importantly to Cd that goes along with it (Friberg and Nordberg 1986). A potential solution is to breed crop cultivars that are more tolerant to high Zn exposure and thus grow relatively well with an acceptable level of Zn accumulation in the leaves.
In Brassica rapa vegetables, an eight, six and 2.5-fold genotypic variation was observed for shoot Zn, Fe and Mn concentration, respectively, and a two-fold variation for relative shoot or root dry biomass production under Zn deficient or toxic conditions (Wu et al. 2007). A two-fold genotypic variation was reported for Ca, Mg, K, Fe, Zn concentration among B. oleracea vegetables (Kopsell et al. 2004; Broadley et al. 2008) and for shoot dry biomass ratio-based Zn efficiency for B. napus and B. juncea (Grewal et al. 1997). The observed natural variation for these traits in Brassica crops suggests the possibility to analyze these traits genetically.
Mineral accumulation in above ground organs is a complex trait controlled by a series of processes, including mobilization from the soil, uptake by the roots, translocation and redistribution within the plant, and import and deposition in the organs (Clemens 2001). This is also the case for plant growth under stressful nutrition conditions because different aspects such as availability, uptake and utilization of nutrient elements can be affected and as a consequence growth, development, and yield of the crop will alter (Gupta 2005). Quantitative trait locus (QTL) mapping allows the identification of individual chromosomal regions containing genetic factors that contribute to variation in a complex trait (Alonso-Blanco and Koornneef 2000). Molecular mapping of B. rapa was initiated by Song et al. (1991) using RFLP markers and a segregating F2 population. Subsequently several additional maps were constructed based on different molecular markers and F2, recombinant inbred lines (RILs) or DH populations (Chyi et al. 1992; Teutonico and Osborn 1994; Kole et al. 1997; Suwabe et al. 2006; Kim et al. 2006; Choi et al. 2007). The recent development of Brassica simple sequence repeat (SSR) markers facilitates the anchoring of linkage groups to one common reference map and allows the comparison of map positions in studies involving different populations (Suwabe et al. 2006; Choi et al. 2007). Furthermore the syntenic relationship with the related genus Arabidopsis is now well established (reviewed by Schranz et al. 2006) and allows the comparison of map positions between Brassica and Arabidopsis. For B. rapa QTL analyses have been described for a wide variety of morphological and physiological traits such as seed colour, pubescence, flowering time (Teutonico and Osborn 1994; Song et al. 1995; Nozaki et al. 1997; Lou et al. 2007), oleic acid concentration (Tanhuanpaa et al. 1996), linolenic acid content (Tanhuanpaa and Schulman 2002), clubroot resistance (Suwabe et al. 2006) and black rot resistance (Sogengas et al. 2007). As microspore culture can be applied efficiently in Brassica species, doubled haploid (DH) populations are presently the preferred mapping populations for QTL studies because of their immortality and homozygosity which allows replicated experiments.
In the present paper we describe the construction of a molecular linkage map containing 203 amplified fragment length polymorphism (AFLP) markers, 58 simple sequence repeat (SSR) markers, 22 sequence related amplified polymorphism (SRAP) markers and four expressed sequence tagged polymorphism (ESTP) markers using 183 DH lines derived from a cross between two Chinese cabbage DH lines. Plants from this population were analyzed for the concentration of 11 elements in leaves, including four essential micro-elements (Fe, Zn, Mn and Cu), five macro-elements (Na, Ca, K, P and Mg), and also for a non-essential element (Sr) and a toxic element (Al). QTL analysis was performed for mineral accumulation and for shoot dry biomass (SDB) yield under normal, deficient and excessive Zn conditions.
Materials and methods
Mapping population and DNA isolation
The BrIVFhn mapping population of 183 DH lines was derived from a cross between two DH Chinese cabbage lines. Y177 originated from a winter type Japanese cultivar ‘Jianchun’ and Y195 is derived from a summer type Chinese cultivar ‘Xiayang’. The two cultivars show differences in bolting time, seed colour, trichome density and flower colour (Supplementary Table 1, Supplementary Fig. 1). DNA from the parents and the DH plants was isolated from the mature leaves as described by Wang et al. (2005).
AFLP analysis
AFLP markers were analyzed following Vos et al. (1995), using fluorescently labelled EcoRI and MseI primers with three selective nucleotides as described by Zhao et al. (2005). AFLPs were scored on the basis of the presence or absence of the band. AFLP markers were named using a code for each EcoRI and MseI primer followed by the band number in ascending molecular-weight order (Table 1).
PCR based markers
A total of 205 SSR markers derived from B. rapa, B. nigra, B. oleracea and B. napus (Lowe et al. 2004; Ge et al. 2005; Suwabe et al. 2002, 2004, 2006; Kim et al. 2006; Choi et al. 2007; T. Osborn, personal communication; G. King personal, communication; G. Bonnema, personal communication) were screened for their polymorphism between the two parental lines. The polymorphic SSR markers with clear bands were used for mapping. Seven Sequence Related Amplified Polymorphism (SRAP) primer combinations (me1/em1, me1/em6, me4/em1, me4/em6, BMe6/BEm12, BMe10/CoEm9, CoMe10/K6), distinguishing the parents, were used to test the DH lines following Li and Quiros (2001). The markers originated from B. oleracea (Li and Quiros 2001), B. napus (Riaz et al. 2001), buffalo grass (Budak et al. 2004) and cotton (Lin et al. 2003). SRAP markers were scored on the basis of the presence or absence of the band and were named using the primer combination followed by a number in descending molecular-weight order. Seven Expressed sequence tagged polymorphism (ESTP) markers (E018, E039, E060, E101, E120, E129, E138) derived from B. rapa cDNA sequences were used to test the population following Choi et al. (2007). PCRs were performed in 20 μl 1 X PCR buffer, containing 20 ng DNA template, 1 U Taq DNA polymerase, 0.25 mM of each dNTP, and 250 nM of each primer. Thermocycling was started at 94°C for 5 min and followed by 35 cycles of 94°C for 1 min, 55°C for 1 min, 72°C for 1 min and a final extension at 72°C for 10 min before holding at 12°C. The PCR products were separated on 6% denaturing polyacrylamide gels and visualized by silver staining.
Segregation analysis and map construction
The segregation of each marker and linkage analysis were performed using JoinMap version 3.0 (http://www.kyazma.nl/). The linkage groups (LGs) were determined using a LOD threshold ≥4.0 and a maximum recombination fraction of 0.4. The Kosambi mapping function (Kosambi 1944) was used to convert recombination frequencies into map distances.
Phenotypic analyses
The leaf mineral concentration was analyzed for the parents and 142 DH lines grown in an open field of the Henan Academy of Agricultural Sciences in Zhengzhou, China in the autumn of 2004. Seeds were first sown in pots (10 cm) with fertilized potting soil. Thirty days after sowing, plants were transplanted to an open field in a randomized two-block design. Soil analysis was carried out according to the method of Agro Services International (ASI) of Orange City, Florida, USA (Table 2). Basal fertilizer (750 kg di-ammonium phosphate per hectare) was applied to plots at the time of transplanting; 375 kg N ha−1 in the form of urea was applied at late rosette stage.
The second fully grown head leaf was harvested from two plants per DH line as two replica, each from a different block, after plants had grown for 30 days in the open field. Harvested leaves were washed with deionized water and lyophilized for 3 days. Samples were ground by mortar and pestle before being ash-digested at 300°C for 1 h and 500°C for 6 h. The digests were dissolved in 1.5 ml 8 M HNO3 and doubled deionized H2O to a final volume of 25 ml. Concentrations of 11 minerals, including Na, Ca, K, P, Mg, Fe, Zn, Mn, Cu, Al and Sr, were determined by inductively coupled plasma—atomic emission spectrometry (ICP-AES; Shimadzu 1000 II, Japan).
To investigate the effect of Zn nutritional stress on shoot dry biomass (SDB) the parental lines and 140 randomly selected DH lines were cultivated hydroponically in a greenhouse without climate control in March (experiment 1: Zn deficiency experiment) and April 2006 (experiment 2: Zn toxicity experiment) in Beijing. The environmental conditions were 15–25°C/8–12°C in March and 20–30°C/10–15°C in April (day/night temperature), 540–720 μmol m−2 s−1 light intensity and 50–60% relative humidity. Half strength Hoagland’s nutrition solution (pH 5.5), buffered with 2 mM MES (2-morpholinoethanesulphonic acid), was used for plant cultivation. Each experiment included a treatment with normal Zn supply (2 μM ZnSO4) and a Zn stress treatment, which was either omitting the addition of ZnSO4 to the medium, to create Zn deficiency, or supplying 100 μM ZnSO4 to create Zn toxicity. In both experiments three replicates were used for both control and Zn stress treatment. Seeds were germinated on agar in 1.5-ml Eppendorf tubes of which the bottom tips had been being cut off and put directly in hydroponic culture trays. Each tray contained 71 DH lines with one plant per line. The trays were shuffled twice a week to reduce a possible effect of location in the greenhouse. After 21 days of growth, whole shoot (aboveground tissue) of each individual was harvested separately and oven-dried at 65°C for 3 days for SDB analysis.
Statistical analysis and QTL mapping
For each DH line, the mean values of 11 mineral concentrations were log10-transformed to improve normality of the distribution. Transformed mineral data were used for QTL analysis. For QTL analysis of SDB under normal Zn supply, data from the two experiments were first standardized, and the mean values of the two experiments were used for QTL analysis. Detection of QTL for SDB under deficient and excessive Zn conditions was conducted with untransformed data. The software package MAPQTL version 5.0 was used to identify and locate QTL on the linkage map by using interval mapping (IM) and multiple-QTL model (MQM) mapping methods as described in the reference manual (http://www.kyazma.nl). A sequential procedure was used for QTL detection. The first step involves finding putative QTLs using IM analysis (Van Ooijen 1992). The significance thresholds accepting the presence of QTLs were determined by permutation tests (1,000 replications; Churchill and Doerge 1994) for each trait at a significance level of α = 0.05. For different traits, the genome wide significance threshold varied between 2.9 and 3.1. Therefore QTLs with a LOD score ≥3.0 were considered to be significant. Markers at these QTLs were taken as cofactors (significant at P < 0.02) to include the effect of the genetic background in MQM analysis (http://www.kyazma.nl). A mapping step size of 1 cM was used for both IM and MQM analyses. The QTL positions were estimated as the position with maximum LOD score on a linkage group. Two-LOD support intervals were established as 95% confidence intervals (Van Ooijen 1992) using MQM mapping implemented with MAPQTL 5.0. For the correlation coefficient (r) test between mineral concentrations for 11 elements, a Bonferroni correction to adjust the 0.05 or 0.01 threshold of significance was applied. Broad sense heritability was estimated for each trait by using the following equation: \(h_b^2 = {{VG} \mathord{\left/ {\vphantom {{VG} {\left( {VG + VE} \right)}}} \right. \kern-\nulldelimiterspace} {\left( {VG + VE} \right)}}\); where VG is the variance between DH lines and VE is the variance within DH lines.
The interaction between the QTLs identified for the same trait was tested by analysis of variance (ANOVA) using the corresponding two markers as fixed factors and the trait as dependent variable at a significance level P ≤ 0.05. For the interaction between genotype and Zn treatment, ANOVA was performed using corresponding markers and Zn treatment as fixed factors and the SDBs as dependent variables. The calculations were carried out using the general linear model module of the SPSS version 12.0.1 statistical package (SPSS Inc., Chicago, IL, USA).
Results
Construction of the BrIVFhn genetic linkage map
Out of the 211 AFLP primer combinations tested on the parental lines, 32 combinations, which each generated over eight polymorphic markers, were selected for genotyping the BrIVFhn mapping population (Table 1). After removing ambiguous markers, in total 202 polymorphic bands were used for mapping. Among these, 110 bands were provided by parent Y177 and 102 by parent Y195. A total of 205 SSR primers were screened for polymorphisms between the parental lines of which 61 displayed a polymorphism and out of these 53 SSRs that could be easily scored using silver stained gels were chosen for genotyping the mapping population. Three of these SSR assays (MAF, OI11B05 and KBRH048011) detected more than one segregating locus. In addition, seven recently reported ESTP markers were screened of which four showed polymorphism between the parental lines. To generate SRAP markers seven primer combinations were used, which amplified two to six polymorphic bands per primer combination in the parents.
In total 287 markers (203 AFLPs, 58 SSRs, 22 SRAPs and four ESTPs) were assigned to 10 linkage groups (LGs) with a LOD score ≥7.0 (Fig. 1). The total length of the map is 1,090 cM, which represents on average one marker for every 3.8 cM. By using the 38 SSRs and four ESTPs with known map positions on the common B. rapa reference map (Lowe et al. 2004; Kim et al. 2006; Suwabe et al. 2006; Choi et al. 2007), the 10 linkage groups were assigned to their corresponding chromosomes R01-R10 (Fig. 1). The individual LGs ranged from 76 cM for R01 and R05 to 145 cM for R09. The number of markers on 10 LGs ranged from 21 (R10) to 41 (R03). A map-interval with markers separated more than 20 cM was only observed on R08. The distribution of markers and the marker density will make this map a useful framework for quantitative trait loci identification.
Based on a χ 2 test for goodness-of-fit to the expected 1:1 Mendelian segregation ratio, skewed segregation was detected for 202 loci (70.3%) at P < 0.05, including 146 AFLP loci, 38 SSR loci, 15 SRAP loci and three ESTP loci. For 154 of the 202 skewed markers the Y195 allele was in excess. Markers that showed skewness were clustered in LGs R01, R07 and R08 and in specific regions on LGs R03, R09 and R10 for markers with an excess of Y195 alleles, and for LGs R02, and R05 this was the case for Y177 alleles (Fig. 1).
Trait analysis
Broad sense heritability of the shoot mineral concentrations in the field experiment was high, ranging from 0.56 for Mg to 0.74 for Mn, respectively (Table 3). Transgression beyond the parental values was observed for nearly all tested elements, including K, Zn and P concentrations for which parental values hardly differed (Table 3; Fig. 2). Differences between DH lines ranged from two-fold for P to 6.5-fold for Fe. In most cases the extent of transgressive variation was towards the lower rather than the higher values. Correlations between mineral concentrations are shown in Table 4. The highest significant correlations were found between Ca, Mg and Sr concentrations, which were 0.84 (Ca/Mg), 0.86 (Ca/Sr) and 0.84 (Mg/Sr) respectively (Table 4). In this population, the Mn concentration was significantly correlated with all other elements, except for K. In all cases significant correlations were positive except for the correlation between Na and K.
The heritability of SDB under different Zn nutritional conditions was lower compared with that of leaf mineral concentrations, with heritability from 0.30 to 0.60. The distribution of the SDB is broad and there is transgression towards lower as well as higher SDB (Table 3). Parental line Y177 has a considerably higher SDB than Y195 under all three tested Zn conditions. On average we found a difference in the SDB of plants growing under normal Zn between experiment 1 and experiment 2, with less biomass for plants in experiment 1, which was carried out earlier in spring. Nevertheless, the correlation of the SDB of DH lines under 2 μM Zn in two experiments was significant (r = 0.43, P ≤ 0.01).
Detection of QTLs
To identify the genetic loci involved in establishing leaf mineral concentration in Chinese cabbage grown in the field and shoot dry biomass production under Zn nutritional stress in hydroponics culture, QTL mapping was performed for the tested 11 minerals and SDB under different Zn nutritional conditions. Ten QTLs were mapped on four LGs for Na, Mg, P, Fe, Mn, Zn, Al and Sr concentrations. No QTL was detected for K, Ca and Cu concentrations in this population (Fig. 1; Table 5). The most significant of the identified QTLs, localizing on R04, explained 17.1% of the Zn concentration variance. Another QTL for Zn was detected on R06, explaining 13.6% of the phenotypic variance. These two QTLs together explained 21.2% of the Zn concentration variance. When tested by ANOVA, no significant interaction was found between the two QTLs. Two QTLs were detected for Mn concentration, one localized on R05 with explained variance of 13.5% and another one localized on R06 with explained variance of 15.7%. The two QTLs together explained 23.5% of the total Mn concentration variance. For the concentrations of Na, Mg, P, Fe, Al and Sr, only one QTL was found for each element. QTLs for Mg and Sr co-localized on R08 and explained 11.9% of Mg and 12.5% of Sr phenotypic variance. Another QTL on R08 explained 10.5% of the Fe concentration variance. A QTL for Na concentration was found on R04, accounting for 16.2% of the phenotypic variance. For P concentration, a QTL was mapped on R06, explaining 11.1% of the phenotypic variance. The QTL associated with Al concentration is located on R05 with an effect of 11.2% of the phenotypic variance.
QTLs related to SDB were identified on R03 and R06. The locus on R03 affects SDB under all three Zn treatments, explaining 14.8%, 15.3% and 12.3%, of the phenotypic variance for SDB under Zn deficiency, normal and excess conditions, respectively. When tested by ANOVA, no significant interactions between genotype and Zn conditions were found for the SDB phenotypic variance at this locus. This suggests that this QTL affects SDB regardless of the Zn supply. The additional QTL on R06 exclusively affected SDB under Zn excess, accounting for 12.6% of the phenotypic variance. No significant interactions between genotype and Zn conditions were found, neither were there significant interactions between the two SDB QTLs.
Discussion
Construction of a B. rapa linkage map
This study reports on the construction of a genetic linkage map for a segregating population of 183 B. rapa DH lines and the first analysis of genetic control of leaf mineral accumulation in B. rapa and shoot dry biomass under different Zn nutrition conditions.
The present linkage map includes 203 AFLP markers, 58 SSR markers, 22 SRAP markers and four ESTP marker grouped on 10 LGs, each anchored to the corresponding chromosome of the B. rapa reference map (Lowe et al. 2004; Kim et al. 2006; Suwabe et al. 2006; Choi et al. 2007) based on common SSR-markers. Our linkage map covers a total genetic distance of 1,090 cM, which compares well with the 1,005.5 and 1,182 cM of two recently published SSR-based maps (Suwabe et al. 2006; Choi et al. 2007) and the 1,287 cM of a sequence-tag-based map (Kim et al. 2006). The number and distribution of the markers over the genome was also comparable to these maps.
A high percentage of skewed markers (70.4%) were observed in our study. This is higher than that of the genetic linkage map based on a DH population of Chinese cabbage (38.3%; Choi et al. 2007), but it is comparable with a proportion of 64% AFLP and RFLP markers deviating from a 1:1 ratio as observed by Voorrips et al. (1997) in a B. oleracea DH mapping population. Skewed segregation ratios have often been observed in populations of doubled haploid plants for many other plant species (Graner et al. 1991), and are most likely due to selection during microspore culture (Foisset et al. 1996). Segregation of skewed markers may generate errors in linkage analysis, resulting in map stretching or a false order of markers on linkage groups. However, simply deleting the markers which show skewed segregation from the map would result in losing all of the skewed segments for trait QTL analysis and thus we decided to include markers with skewed segregation in the map.
QTLs for mineral accumulation
We analyzed leaf mineral concentration in the mapping population and found transgression for all 11 elements. Nevertheless, no QTL was detected for three of these elements including K, which showed transgressive variation to both sides of the parental values. The failure to detect QTLs associated with transgressed traits was previously reported for RIL populations of tomato (Saliba-Colombani et al. 2001) and tobacco (Julio et al. 2006). Transgressive segregation in a population is normally due to the presence of complementary QTL alleles in the two parental lines. However if there are several QTLs and the QTL effects are relatively small they may not be detected.
The trait analysis showed significant positive correlations among some of the tested minerals, including toxic element Al and non-essential element Sr. This was also the case for seed mineral content in common bean (Beebe et al. 2000) and Arabidopsis (Vreugdenhil et al. 2004). The correlation between different minerals implicated pleiotropy for genes controlling accumulation of these minerals or close linkage of genes. Therefore consideration must be taken when designing a breeding program for improvement of mineral concentrations, especially to avoid accumulation of toxic minerals. However, we did not find as many co-localized QTLs as we found significant correlations between concentrations of different minerals. This could be due to a large number of QTLs involved in mineral accumulation but each with minor effect and therefore is difficult to be detected. Co-localization of QTLs involved in different minerals was reported previously for Arabidopsis seed mineral content with most of the co-localizations of K/Ca and K/Ca/Mn QTLs (Vreugdenhil et al. 2004) and recently for Brassica oleracea shoot Ca/Mg concentrations (Broadley et al. 2008). Although we found strong correlation between Mg, Ca and Sr concentrations, we only found QTLs for Mg and Sr, but these were the only mineral QTLs that co-localized in the studied population. Although it has been reported that there is no selectivity or interactions between Ca and Sr for transport to the shoots (reviewed by White 2001), the correlation between the concentration of these minerals and the co-location of QTLs indicates that the accumulation of Ca, Mg and Sr in shoots might share a common mechanism. This was also supported by a suggestive QTL in the same region of QTLs on R08 for Ca, with a peak of LOD = 2.42. R08 shares high level of co-linearity with the chromosome C08 of B. oleracea (Parkin et al. 2005), on which Broadley et al. (2008) identified co-localized QTLs for shoot Mg and Ca concentrations. This provides clue that homologus genes in B. rapa and B. olearacea are likely being involved in Mg and Ca accumulation. However, as no common anchoring marker was used in these two studies, further clarification is needed to prove the alignment of these QTLs for Mg accumulation in the two species.
While the heritabilities for most mineral concentrations were high, only one or two QTLs were detected for individual minerals, with a relatively low percentage of explained variance per locus varying from 10.5–17.1%. This means that many QTLs remained undetected, probably because of small effects of each QTL. This underlines the complex genetic control of leaf mineral accumulation in this population. If this is common in B. rapa it will be very difficult to set up an efficient breeding program for improved leaf mineral concentrations. For this population, the parents were not very different in terms of leaf mineral concentrations. Previous work from our group on Fe, Mn and Zn leaf concentrations (Wu et al. 2007) showed that accessions with larger differences can be found in B. rapa germplasm. Choosing such accessions as parents of a segregating population could simplify the genetic complexity and allow identification of more QTLs.
QTL for SDB
We carried out two independent experiments for plant SDB analysis under Zn deficiency and Zn excess conditions. Relative shoot growth based on dry biomass was previously identified as a suitable parameter for tolerance evaluation of Brassica crops to Zn stress (Grewal et al. 1997; Wu et al. 2007). Therefore in the present study we investigated SDB under deficient and excess Zn supply. Considering that SDB normally represents a complex trait including production-related characteristics as well as adaptive characteristics that must be changed in plants in order to adapt to (a)biotic stress (Ronnberg-Wastljung and Gullberg 1999), we also analyzed SDB under normal Zn supply to be able to distinguish general SDB QTLs from stress-specific SDB QTLs. Only a few QTLs were detected for SDB, with low explained variance (≤15%). This is consistent with previous reports that the analyses of plant responses to environmental stress generally reveal only few major QTL (Koyama et al. 2001), again indicating that a large number of genes contribute to the overall phenotype.
A QTL for SDB was mapped on R03 under different Zn nutrition conditions. It did not show a significant interaction between the genotype of this locus and the Zn treatment, thus this locus controls plant SDB in general. Also for the Zn100SDB6 QTL on R6, which was identified for excessive Zn only, the interaction between genotype and Zn condition was not significant. As the LOD score of this locus, with a low explained variance, was just above the threshold for QTL determination, such minor QTL could have escaped QTL detection under normal and Zn deficient conditions. Inefficient detection of SDB QTLs under Zn stress conditions, as in the present study, is most likely due to the multigenic inheritance of the trait, which has also been reported for QTL mapping of rice tolerance to Zn deficiency (Wissuwa et al. 2006). More detailed physiological studies that distinguish between sub-processes are likely to improve genetic dissection on tolerance to Zn stress. Also the much higher effect of Zn condition (20.9%) on SDB than that of genotype of this locus (4.5%), as revealed by ANOVA, indicates that genetic improvement on Zn stress tolerance will need integration of a large number of genes.
Abbreviations
- AFLP:
-
amplified fragment length polymorphism
- DH:
-
doubled haploid
- ESTP:
-
expressed sequence tagged polymorphism
- MQM:
-
multiple-QTL model
- QTL:
-
quantitative trait locus
- SDB:
-
shoot dry biomass
- SRAP:
-
sequence related amplified polymorphism
- SSR:
-
simple sequence repeat
References
Alonso-Blanco C, Koornneef M (2000) Naturally occurring variation in Arabidopsis: an underexploited resource for plant genetics. Trends Plant Sci 5:387–391
Assunção AGL, Pieper B, Vromans J, Lindhout P, Aarts MGM, Schat H (2006) Construction of a genetic linkage map of Thlaspi caerulescens and quantitative trait loci analysis of zinc accumulation. New Phytol 170:21–32
Banziger M, Long J (2000) The potential for increasing the iron and zinc density of maize through plant breeding. Food Nutr Bull 21:397–400
Beebe S, Gonzalez AV, Rengifo J (2000) Research on trace minerals in the common bean. Food Nutr Bull 21:387–391
Bentsink L, Yuan K, Koornneef M, Vreugdenhil D (2003) The genetics of phytate and phosphate accumulation in seeds and leaves of Arabidopsis thaliana, using natural variation. Theor Appl Genet 106:1234–1243
Bouis H (2002) Plant breeding: a new tool for fighting micronutrient malnutrition. J Nutr 132:491S–494S
Broadley MR, Hammond JP, King GJ, Astley D, Bowen HC, Meacham MC, Mead A, Pink DAC, Teakle GR, Hayden RM, Spracklen WP, White PJ (2008) Shoot calcium (Ca) and magnesium (Mg) concentration differ between subtaxa, are highly heritable, and associated with potentially pleitropic loci in Brassica oleracea. Plant Physiol 146:1707–1720
Budak H, Shearman R C Parmaksiz I, Gaussoin RE, Riordan TP, Dweikat I (2004) Molecular characterization of buffalograss germplasm using sequence-related amplified polymorphism markers. Theor Appl Genet 108:328–334
Choi SR, Teakle GR, Plaha P, Kim JH, Allender CJ, Beynon E, Piao ZY, Soengas P, Han TH, King GJ, Barker GC, Hand P, Lydiate DJ, Batley J, Edwards D, Koo DH, Bang JW, Beom-Seok P, Lim YP (2007) The reference genetic linkage map for the multinational Brassica rapa genome sequencing project. Theor Appl Genet 115:777–792
Churchill GA, Doerge RW (1994) Empirical threshold values for quantitative trait mapping. Genetics 138:963–971
Chyi YS, Hoenecke ME, Sernyk JL (1992) A genetic map of restriction fragment length polymorphism loci for Brassica rapa (syn. campestris). Genome 35:746–757
Clemens S (2001) Molecular mechanisms of plant metal tolerance and homeostasis. Planta 212:475–486
Deniau AX, Pieper B, Ten Bookum WM, Lindhout P, Aarts MGM, Schat H (2006) QTL analysis of cadmium and zinc accumulation in the heavy metal hyperaccumulatior Thlaspi caerulescens. Theor Appl Genet 113:907–920
Foisset N, Delourme R, Barret P, Hubert N, Landry BS, Renard M (1996) Molecular mapping analysis in Brassica napus using isozyme, RAPD and RFLP markers on a double haploid progeny. Theor Appl Genet 93:1017–1025
Friberg L, Nordberg GF (1986) Introduction. In: Friberg L, Nordberg GF, Vouk VB, Kessler E (eds) Handbook on the toxicity of metals, 2nd edn. Elsevier Science BV, Amsterdam, The Netherlands, pp 1–14
Ge J, Xie H, Cui CS, Hong JM, Ma RC (2005) Analysis of expressed sequence tags (ESTs) derived SSR markers in Chinese cabbage (Brassica campestris L. ssp. pekinensis). J Agric Biotech 13:423–428
Ghandilyan A, Vreugdenhil D, Aarts MGM (2006) Progress in the genetic understanding of plant iron and zinc nutrition. Physiol Plant 126:407–417
Graner A, Jahoor A, Schondelmaier J, Siedler H, Pillen K, Fischbeck G, Wenzel G, Herrmann RG (1991) Construction of an RFLP map of barley. Theor Appl Genet 83:250–256
Gregorio GB, Senadhira D, Htut H, Graham RD (2000) Breeding for trace mineral density in rice. Food Nutr Bull 21:382–386
Grewal HS, Stangoulis JCR, Potter T, Graham RD (1997) Zinc efficiency of oilseed rape (Brassica napus and B. juncea) genotypes. Plant Soil 191:123–132
Gupta US (2005) Physiology of stressed crops, volume II. Nutrient relations. Science Publishers INC, Enfield, NH, USA, pp 1–25
Hacisalihoglu G, Kochian LV (2003) How do some plants tolerate low levels of soil zinc? Mechanisms of zinc efficiency in crop plants. New Phytol 159:341–350
Harada H, Leigh RA (2006) Genetic mapping of natural variation in potassium concentrations in shoots of Arabidopsis thaliana. J Exp Bot 57:953–960
Islam F, Basford KE, Jara C, Redden RL, Beebe S (2002) Seed compositional and disease resistance difference among gene pools in cultivated common bean. Genet Resour Crop Evol 49:258–293
Julio E, Denoyes-Rothan B, Verrier J-L, Dorlhac de Borne F (2006) Detection of QTLs linked to leaf and smoke properties in Nicotiana tabacum based on a study of 114 recombinant inbred lines. Mol Breed 18:69–91
Kim JS, Chung TY, King GJ, Jin M, Yang T, Jin Y, Kim H, Park B (2006) A sequence-tagged linkage map of Brassica rapa. Genetics 174:29–39
Kole C, Kole P, Vogelzang R, Osborn TC (1997) Genetic linkage map of a Brassica rapa recombinant inbred population. J Heredity 88:553–557
Kopsell DE, Kopsell DA, Lefsrud MG, Curran-Celentano J (2004) Variability in elemental accumulations among leafy Brassica oleracea cultivars and selections. J Plant Nutr 27:1813–1826
Kosambi DD (1944) The estimation of map distance from recombination values. Ann Eugen 12:172–175
Koyama ML, Levesley A, Koebner RMD, Flowers TJ, Yeo AR (2001) Quantitative trait loci for component physiological traits determining salt tolerance in rice. Plant Physiol 125:406–422
Li G, Quiros CF (2001) Sequence-related amplified polymorphism (SRAP), a new marker system based on a simple PCR reaction: its application in mapping and gene tagging in Brasisca. Theor Appl Genet 103:455–461
Lin Z, Zhang X, Nie Y, He D, Wu M (2003) Construction of a genetic linkage map for cotton based on SRAP. Chin Sci Bull 48:2063–2067
Liu W, Zhao J, Ouyang Z, Soderlund L, Liu G (2005) Impacts of sewage irrigation on heavy metal distribution and contamination in Beijing China. Environ Int 31:805–812
Lou P, Zhao JJ, Kim JS, Shen SX, Del Carpio DP, Song XF, Jin M, Vreugdenhil D, Wang XW, Koornneef M, Bonnema G (2007) Quantitative trait loci for flowering time and morphological traits in multiple populations of Brassica rapa. J Exp Bot 58:4005–4016
Lowe AJ, Moule C, Trick M, Edwards KJ (2004) Efficient large-scale development of microsatellites for marker and mapping applications in Brassica crop species. Theor Appl Genet 108:1103–1112
Ma G, Li Y, Jin Y, Du S, Kok FJ, Yang X (2007) Assessment of intake inadequacy and food source of zinc of people in China. Public Health Nutr 10:848–854
Monasterio I, Graham RD (2000) Breeding for trace minerals in wheat. Food Nutr Bull 21:392–396
Nan ZR, Zhao CY (2000) Heavy metal concentrations in grey calcareous soils of Baiyin region, Gansu Province, P.R.China. Water Air Soil Pollut 118:131–141
Nozaki T, Kumazaki A, Koba T, Ishikawa K, Ikehashi H (1997) Linkage analysis among loci for RAPDs, isozymes and some agronomic traits in Brassica campestris L. Euphytica 95:115–123
Payne KA, Bowen HC, Hammond JP, Hampton CR, Lynn JR, Mead A, Swarup K, Bennett MJ, White PJ, Broadley MR (2004) Natural genetic variation in caesium (Cs) accumulation by Arabidopsis thaliana. New Phytol 162:535–548
Parkin IA, Gulden SM, Sharpe AG, Lukens L, Trick M, Osborn TC, Lydiate DJ (2005) Segmental structure of the Brassica napus genome based on comparative analysis with Arabidopsis thaliana. Genetics 171(2):765–81
Riaz A, Li G, Quresh Z, Swati MS, Quiros CF (2001) Genetic diversity of oilseed Brassica napus inbred lines based on sequence-related amplified polymorphism and its relation to hybrid performance. Plant Breed 120:411–415
Ronnberg-Wastljung AC, Gullberg U (1999) Genetics of breeding characters with possible effects on biomass production in Salix viminalis. Theor Appl Genet 98:531–540
Saliba-Colombani V, Causse M, Langlois D, Phiouze J, Buret M (2001) Genetic analysis of organoleptic quality in fresh market tomato: 1. Mapping QTLs for physical and chemical traits. Theor Appl Genet 102:259–272
Schranz ME, Lysak MA, Mitchell-Olds TM (2006) The ABC’s of comparative genomics in the Brassicaceae: building blocks of crucifer genomes. Trends Plant Sci 11:535–542
Sogengas P, Hand P, Vicente JG, Pole JM, Pink DAC (2007) Identification of quantitative trait loci for resistance to Xanthomonas campestris pv. campestris in Brassica rapa. Theor Appl Genet 114:637–645
Song KM, Suzuki JY, Slocum MK, Williams PH, Osborn TC (1991) A linkage map of Brassica rapa (syn. campestris) based on restriction fragment length polymorphism loci. Theor Appl Genet 82:296–304
Song KM, Slocum MK, Osborn TC (1995) Molecular marker analysis of genes controlling morphological variation in Brassica rapa (syn. campestris). Theor Appl Genet 90:1–10
Suwabe K, Iketani H, Nunome T, Kage T, Hirai M (2002) Isolation and characterization of microsatellites in Brassica rapa L. Theor Appl Genet 104:1092–1098
Suwabe K, Iketani H, Nunome T, Ohyama A, Hirai M, Fukuoka H (2004) Characteristics of microsatellites in Brassica rapa genome and their potential utilization for comparative genomics in Cruciferae. Breed Sci 54:85–90
Suwabe K, Tsukazaki H, Iketani H, Hatakeyama K, Kondo M, Fujimura M, Nunome T, Fukuoka H, Hirai M, Matsumoto S (2006) Simple sequence repeat-based comparative genomics between Brassica rapa and Arabidopsis thaliana: the genetic origin of clubroot resistance. Genetics 173:309–319
Tanhuanpaa PK, Vilkki JP, Vilkki HJ (1996) Mapping of a QTL for oleic acid concentration in spring turnip rape (Brassica rapa ssp. oleifera). Theor Appl Genet 92:952–956
Tanhuanpaa P, Schulman A (2002) Mapping of genes affecting linolenic acid content in Brassica rapa ssp. oleifera. Mol Breed 10:51–62
Teutonico RA, Osborn TC (1994) Mapping of RFLP and quantitative trait loci in Brassica rapa and comparison to the linkage maps of B. napus, B. oleracea and Arabidopsis thaliana. Theor Appl Genet 89:885–894
Vallee BL, Auld DS (1990) Zinc coordination, function, and structure of zinc enzymes and other proteins. Biochemistry 29:5647–5659
Van Ooijen JW (1992) Accuracy of mapping quantitative trait loci in autogamous species. Theor Appl Genet 84:803–811
Voorrips RE, Jongerius MC, Kanne HJ (1997) Mapping of two genes for resistance to clubroot (Plasmodiophora brassicae) in a population of doubled haploid lines of Brassica oleracea by means of RFLP and AFLP markers. Theor Appl Genet 94:75–82
Vos P, Hogers R, Bleeker M, Reijans M, Van de Lee T, Hornes M, Friters A, Pot J, Peleman J, Kuiper M, Zabeau M (1995) AFLP: a new technique for DNA fingerprinting. Nucleic Acids Res 23:4407–4414
Vreugdenhil D, Aarts MGM, Koornneef M, Nelissen H, Ernst WHO (2004) Natural variation and QTL analysis for cationic mineral content in seeds of Arabidopsis thaliana. Plant Cell Environ 27:828–839
Wang XW, Lou P, Bonnema G, Yang BJ, He HJ, Zhang YG, Fang ZY (2005) Linkage mapping of a dominant male sterility gene Ms-cd1 in Brasscia oleracea. Genome 48:848–854
White PJ (2001) The pathway of calcium movement to the xylem. J Exp Bot 358:891–899
Wissuwa M, Ismail AM, Yanagihara S (2006) Effect of Zn deficiency on rice growth and genetic factors contributing to tolerance. Plant Physiol 142:731–741
Wu J, Schat H, Sun RF, Koornneef M, Wang XW, Aarts MGM (2007) Characterization of natural variation for zinc, iron and manganese accumulation and zinc exposure response in Brassica rapa L. Plant Soil 291:167–180
Zhao JJ, Wang XW, Deng B, Lou P, Wu J, Sun RF, Xu ZY, Vromans J, Koornneef M, Bonnema G (2005) Genetic relationships within Brassica rapa as inferred from AFLP fingerprints. Theor Appl Genet 110:1301–1314
Acknowledgements
We thank Dr. T Osbon, Dr. G King and Dr. G Bonnema for the information on SSR markers. We are grateful to Joost Keurentjes for his help on data analyses. The work was supported by National Basic Research and Development Program (2006CB101606), National 863 High Technology Program, P.R. China (2006AA100108), The Opening Lab of Vegetable Genetics and Physiology of the Ministry of Agriculture, P.R. China and the Interdisciplinary Research and Educational Fund (INREF) of Wageningen University, the Netherlands. The research was conducted at the Sino-Dutch Joint Plant Genome Analysis Laboratory at the Institute of Vegetables and Flowers (IVF-CAAS) in Beijing.
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Jian Wu and Yuxiang Yuan contributed equally.
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Wu, J., Yuan, YX., Zhang, XW. et al. Mapping QTLs for mineral accumulation and shoot dry biomass under different Zn nutritional conditions in Chinese cabbage (Brassica rapa L. ssp. pekinensis). Plant Soil 310, 25–40 (2008). https://doi.org/10.1007/s11104-008-9625-1
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DOI: https://doi.org/10.1007/s11104-008-9625-1