Abstract
Due to several reasons soil-borne viruses such as the furoviruses, i. e., cereal mosaic virus (SBCMV) and wheat mosaic virus (SBWMV) as well as the bymovirus wheat spindle streak mosaic virus (WSSMV) gained importance in cereal breeding including rye. High yield losses are recorded, today. Since there is no or little resistance to these viruses in modern rye cultivars, an extended screening for resistance was initiated. In addition to earlier screenings, 37 rye genotypes were tested for resistance. Among them, three genotypes were found with persistent resistance to SBCMV. They belong to Secale montanum and S. vavilovii species, i. e., wild types of rye. One accession, PC2243 (S. montanum), was used as a resistance donor for the present genetic study. In F2 generation, it was observed that resistance to SBCMV is independently inherited from WSSMV. The evaluation of the ELISA values pointed to a 3:1 distribution assuming duplicate dominant epistasis. Molecular marker analysis supports this segregation pattern. By composite interval mapping a QTL on chromosome 2R could be detected. It can be assumed that there is a DNA region of about 13 cM on the long arm of chromosome 2R (2RL) harboring SBCMV resistance with the closest markers “C9654_1947” and “isotig11640”. Moreover, genotypes with a yellow seed coat showed practically no infection with SBCMV. Thus, the resistance gene could be linked to the allele an1 determining non expression of anthocyanins. This locus was also mapped earlier on chromosome 2R.
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Introduction
Since centuries cereals including rye are major crops, particularly in Europe, for feeding, bread making and as renewable resources. Rye cropping on poor, sandy soils and restricted crop rotations promote the growth of soil-borne viruses such as the furovirus cereal mosaic virus (SBCMV) and wheat mosaic virus (SBWMV) as well as the bymovirus wheat spindle streak mosaic virus (WSSMV, see Table 1). Global warming may contribute to the increasing spread of these viruses in the temperate zones of Europe. In the affected areas, yield losses in grain of up to 70% are recorded, at least in wheat (Budge et al. 2008).
Both SBCMV and WSSMV are vectored by the obligate biotrophic root parasite Polymyxa graminis (Kanyuka et al. 2003). As spores of P. graminis persist in the soil and soil-borne viruses remain viable therein for decades, susceptible cereals cannot be grown on infested fields (Driskel et al. 2004). Because neither chemical control of virus and the respective vector nor crop rotation is effective, breeding of resistant varieties seems to be the only way of plant protection (Ordon et al. 2009).
Since there is no resistance to these viruses present in modern rye varieties, an extended screening for resistant genotypes was initiated years ago (Huth et al. 2007; Kastirr et al. 2006, 2011, 2012; King et al. 2011; Kühne 2009; Ziegler et al. 2015). Only Cadle-Davidson et al. (2006) identified the old U.S. American rye variety “Aroostook” being resistant to WSSMV. However, respective results could not be confirmed under German growing conditions (U. Kastirr, personal comm., 2016), maybe due to the genetic heterogeneity of the samples used.
Erath et al. (2016) tested more than 500 accessions of Secale cereale and S. montanum from 48 different geographical regions in growth chambers with virus-infested soil. Within these genetic resources 35 accessions were detected with a lower infection rate and low virus titre. These genotypes were cultivated on infested fields of five different environments. Two of these regions were mix contaminated by SBCMV and WSSMV and three fields respectively only by SBCMV, SBWMV, and WSSMV. Just one rye population, derived from the combination S. cereale var. Lo86 x S. cereale var. Moor-Roggen led to a more detailed segregation analysis of F2 to F6 populations showing moderate resistance controlled by quantitative trait loci (QTL) on chromosome 5R (SBCMV) and 7R (WSSMV).
In order to extent search for resistant rye genomes, in 2012 an additional screening was initiated considering genetic tester stocks, wheat-rye amphiploids, and related wild species of rye. Because of the high degree of genetic variability within the populations, supposedly resistant plants were isolated and used for crosses and resistance testing by ELISA. Three genotypes out of 37 turned out to be persistently resistant to SBCMV. The accession PC2243 from Secale montanum was used as a resistance donor for the present genetic study.
Materials and methods
Plant material
Out of the cytogenetic tester tsock collection (curator R. Schlegel, 1971–2020), 37 genotypes of a wide range of rye genomes were tested for resistance to soil-borne viruses: diploid S. cereale var. Imperial, var. Insave, var. Maton (USA, WSMV res.), var. Petkuser, var. Rosen (Russia > USA), str. Lochow 120-P, str. Lochow KWL1, inbred line; diploid S. montanum str. R797, str. R2501 (UK); diploid S. cereale var. (unknown origin, Quedlinburg); tetraploid S. cereale var. Gorzow, var. Shitomirskaja, var. Sopronyhorpacsi, var. Ukrainskaja, str. 3551/70, str. 3130/69; diploid S. africanum str. R1210, diploid; 2Rafr(2D) wheat-rye substitution, T. aestivum x S. africanum (kindly provided by Zujun Yang, Chengdu, China); S. vavilovii, collected Armenia by the author; S. cereale, var. Heines Hellkorn, Trisomic 1R…7R (kindly provided by F. J. Zeller, Weihenstephan, Germany); rye-wheat addition 5D, from S. cereale var. Pluto x T. aestivum var. Fakon; hexaploid Triticum turgidocereale var. Pika, BBAARR; amphi-octoploid Triticum rimpauii, T. aestivum var. Chinese Spring x S. montanum, BBAADDRR, var. T. aestivum var. Chinese Spring x S. cereale var. Imperial, var. T. aestivum var. Chinese Spring x S. cereale var. King II, BBAADDRR; var. T. aestivum var. Azle x S. cereale var. Pearl; Wheat-rye addition 1Rmo, 2Rmo, 4Rmo, 5RSmo and 6Rmo T. aestivum var. Chinese Spring–S. montanum, 2n = 44.
Four mapping populations segregating for SBCMV and WSSMV were established from combinations (a) Secale cereale var. Imperial x S. montanum, (b) S. cereale var. Imperial x S. africanum, (c) S. cereale var. Inbred line (KWL1) x S. montanum, and (d) S. cereale var. Imperial x S. vavilovii. However, in this paper the first of the four combinations (a) is considered only, and exclusively for SBCMV.
After crossing and production of F1 plan ts two mapping populations of 202 and 133 F2 plants were established, resp. The individual seedlings, separated by four classes of different seed color (cf. Table 4), were planted in September 2018 on a SBCMV- and WSSMV-infested field plot at Thören (Lower Saxony). In addition, a replicated population with 133 plants was used for planting in September 2019 on a SBCMV- and WSSMV-infested field at Walternienburg (Saxony-Anhalt). Because of the high degree of phenotypic variation and mild symptom development, no phenotypic trait assessment was performed.
ELISA
The virus concentration in parents and progeny was determined by semi-quantitative DAS-ELISA (double antibody sandwich enzyme-linked immunosorbent assay) according to Clark and Adams (1977). In March 2019 and March 2020, the youngest leaves of plants were collected. The extracted leaf sap from 0.1 g leaf tissue was diluted 1:20 with extraction buffer and added to microtitre plate wells (Nunc Maxisorp, San Diego, CA, USA), which were coated with specific antibodies against SBCMV or WSSMV, respectively. The extinction (optical density, OD) was measured at 405 nm.
DNA extraction and molecular analysis
Genomic DNA was extracted from F2 plants including parental individuals with a silica-membrane technology according to a Macherey & Nagel NucleoSpin 96 Plant II DNA extraction kit (Saghai-Maroof et. al. 1984, Anonymous 2019a).
Marker data were obtained by using a KWS custom 10 k Infinium iSelect single nucleotide polymorphism (SNP) array according to the supplier guidelines. From the array, public available markers (Martis et al. 2013; Bauer et al. 2017) have been used in combination with a KWS internal combined genetic map.
QTL analysis was conducted with R (R Core Team, Anonymous 2019b) using the library R-QTL (Broman et al. 2003). Markers were removed by using a minor allele frequency of 1% and if they had more than 50% missing data. Only one marker was kept in case of co-segregation. Individuals with more than 50% missing data after marker QC were removed. Phenotypic values of parental components were not considered.
Reported QTL detecting methods are SIM and CIM. Both approaches use a genetic map, in contrast to single marker regression (results not shown). SIM (simple interval mapping) scans for QTL between adjacent markers with the drawback that markers outside the interval can influence the result, e.g., caused by genetic background. CIM (composite interval mapping) includes the genetic background by applying intervals with cofactors used as regressors.
Results
Screening for new sources of resistance
Over eight years, 37 different rye genomes from distant gene pools were examined. It was carried out both under controlled conditions in the greenhouse and mostly in fields that are contaminated with the various viruses, which were characterized in several reports (Kastirr 2004; Kastirr und Ziegler 2018). However, those test sites showed great variability in the infestation of cereal plants. Of course, this made genetic analysis more difficult (see Table 2).
The results obtained over the years are summarized in Table 2. Since sometimes rye populations classified to be resistant had to be declared as susceptible at other testing locations, it was extremely difficult to select suitable populations with virus resistance for a subsequent genetic analysis.
In the case of rye, three accessions turned out to be resistant after repeated studies, i.e., the wild rye Secale montanum (PC2243), S. africanum (PC2328), and S. vavilovii (PC2364). Since the allogamous rye generally has a high degree of genetic variability, the three isolated populations were further separated and increased by self-pollination. Among the cultivated rye, S. cereale, no resistant source was identified during these studies (cf. Table 2).
Virus infestation
Leaf symptoms (cf. Figure 1) of SBCMV could not be estimated in all plants, however, sporadically. Therefore, ELISA was used as main criterion for virus infestation of tillering plants. During ELISA testing the titre threshold was set to 0.1 to characterize infected plants. On the test site Thören, in 2019 there was little infestation for WSSMV that even the parental lines of S. cereale var. Imperial and S. montanum did not show any reaction (Table 3). It was decided to only consider the infestation with SBCMV.
The first comparison of the viral infestation of young plants showed that the WSSMV did not cause any significant symptoms at the chosen location of Thören. Even the parental genotypes PC272 and PC2243 did not differ (Table 3). The F2 analysis at the Thören location was therefore not suitable for the WSSMV study and was thus no longer considered. However, some plants were found to be susceptible to WSSMV, but not to SBCMV. This means that the susceptibility or resistance is independently determined for WSSMV and SBCMV.
SBCMV
The evaluation of the ELISA values shows that in 2019 19 of the 170 genotyped plants exhibit a clear infection to SBCMV and 151 none. (Table 4). When this distribution of 151r: 19s is compared to a 3r:1s expectation (= 127.5r: 42.5s), then just a slight association can be considered. However, the observed distribution matches better with a 9:3:3:1 or 15r:1s distribution (= 159.4r: 10.6s) assuming duplicate dominant epistasis, suggesting A epistatic to B and b, B epistatic to A and a.
The statistical analysis applying Chi2 test did not clearly confirm neither a 3r:1s nor a 15r:1s distribution (cf. Table 5 and 6) in 2019. By the Chi2 values of 17.32 (3r:1s) and 7.03 (15r:1s) the null hypothesis can be rejected within the confidence level of P = 0, df = 1 and P = 0.0081, df = 1, respectively.
However, when false-negative plants taken into account that occur with about 10% and more in 2019, then the Chi2 values change to Chi2 = 2.3, P = 0.1294, for a 3r:1s segregation and Chi2 = 51.84, P = 0, for 15r:1s segregation. Because of various environmental conditions and inhomogeneous Polymyxa spatial distributions false-negative plants are always found in these field trials. Thus, a Chi2 value of 2.3 (P = 0.1294, df = 1) would indicate a 3r:1s segregation rather than a 15r:1s, respectively. This suggestion fits to the replication of the study in 2020 with a more homogenous virus infestation as well as the molecular study.
Mapping analysis
Based on the ELISA scores given in Table 4 the molecular data were associated with the phenotypic result. The prerequisite for this study was a clear differentiation of the ELISA scores for SBCMV between the parents PC272 and PC2243 (cf. Figure 2).
Altogether 8,950 molecular markers were available, from which 6,362 were mapped across the seven rye chromosomes. For the study on SBCMV totally 987 cleaned and translatable markers were included: 1R = 133, 2R = 135, 3R = 133, 4R = 162, 5R = 200, 6R = 152, 7R = 72, i. e., about 141 per chromosome. With the exception of chromosome 7R, there is a balanced distribution across the genome (cf. Fig. 3).
Applying these 987 markers and composite interval mapping (CIM) a QTL on chromosome 2R was detected (cf. Table 7 and Fig. 4). In this comparison, the phenotypic results of the parents were not included because of the allele effects that are highly influenced by the A-parent (S. cereale var. Imperial). The differences for the allele frequencies between groups are larger or smaller 0.1, i.e., they are rather small (Table 7).
Taking all restrictions into account, it can be assumed that there is a genetic stretch of about 13 cM (between 114 and 127 cM) on the long arm of chromosome 2R critical for the SBCMV resistance in this particular population (Fig. 4). The markers “C9654_1947” and “isotig11640” are the peak markers within this region (Table 7).
Additional calculations, such as a reduced ABH matrix with expected segregation patterns only or transformed phenotypes, where scores larger 0.1 have been coded as 1 and smaller 0.1 as 0 to simulate the non-linearity and/ or sensitivity of the ELISA test, did not improve the significance of the results. The application of the basic local alignment search tool (BLAST) for known wheat markers to SBCMV did not show a clear overlapping with the detected region on 2R. The molecular investigation also revealed a higher heterozygosity for the donor parent S. montanum as compared to the recipient parent "Imperial" (Table 7) that is in general agreement with morphological observations.
This can be explained by the fact that the variety "Imperial" variety has been propagated over several generations through self-pollination, while the S. montanum accession resulted from a sample that was once collected with two multiplications under isolated conditions.
Variation of seed color
It is known that the color of the rye caryopses can vary from yellow, green, brown to violet (Schlegel 2013). In the present investigation, the female cross parent “Imperial” had green and the male parent, S. montanum, brownish grains. The F1 grains were dark green throughout. But in the F2 generation there was a clear segregation of the seed color.
Therefore it seemed reasonable to consider this phenotypic variation in relation to the resistance against SBCMV.
Thus, four groups of approximately the same size were created for the colors yellow, green, green-yellow, and brown (cf. Fig. 5). They were sown separately and later compared with the ELISA results. Plants susceptible to SBCMV (ELISA scores > 0.10) occur with different frequencies between the classes of seed color (Table 4) and can be distinguished if the ELISA scores of the four groups are averaged. The highest ELISA scores are found among the green-yellow and brown-colored seeds. These differences from the purely yellow and green seeds are statistically significant (Tables 8, 9 and 10). It shows that the plants with the yellow seed coat show practically no infection with SBCMV.
Discussion
Screening
Both earlier screenings of rye genomes and the current study indicate that little genetic variability can be expected in adapted rye (Secale cereale), although rye generally shows a high degree of variability as it is a typical open-pollinator. The first studies by Erath et al. (2016) as well as the present results show that significant resistance can only be found in wild rye, particularly in the perennial Secale montanum and S. africanum as well as within the annual S. vavilovii. While S. montanum and S. africanum belong to the genome complex of S. strictum, S. vavilovii syn. S. ranicum are declared to be part of the S. cereale genome complex (Hammer et al. 1987). Further screenings should therefore focus on accessions from these genome complexes. However, this does not render breeding of resistant rye varieties easier. The critical genes have first to be transferred to the modern varieties and/or inbred lines via laborious introgressions and back crosses. However, the results indicate a monogenic, dominant inheritance, which is favorable for hybrid rye breeding.
Molecular study
As stated above, it is likely that the molecular markers “C9654_1947” and “isotig11640” on chromosome 2RL are closely linked to resistance against SBCMV. The region covers about 14 cM of the DNA and segregates according to a monogenic mode of inheritance. In order to support this assumption, the investigation of a corresponding physical stretch of around 30 Mbp is recommended to detect a candidate gene and/or genes. For a repeated study, the population size should be enlarged to increase the chance for susceptible individuals. The precision of the ELISA testing together with an optimized experimental design toward uniform SBCMV infestation may contribute to this approach.
Cytological studies should also be involved because the donor genome of Secale montanum differs by two reciprocal translocations involving the chromosomes 2R, 6R, and 7R (cf. Figure 6). In F1 plants, a hexavalent chromosome configuration is usually formed during metaphase I of meiosis. This may lead to a non-regular distribution of chromosomal segments in F2 generation and can make the chromosomal assignment of the markers difficult.
Also in the experiment carried out by Erath et al. (2016), no resistance genes have so far been identified that can be used in rye breeding. Additional characterization of the DNA segment on chromosome 2R therefore offers the chance to describe such a gene and to create suitable markers for it.
Seed color
The color of the rye grains depends on the combination of the color, thickness, and transparency of the seed coat (pericarp), and of the color of the aleuron layer. It may vary between bright yellow, dark yellow, bright red-brown, brown, dark brown, and violet. Rye with brown and black grains or seeds with brown tips are not suitable for practical utilization. Steglich and Pieper (1922) were the only ones who described black xenia in crosses with “Pirnaer Roggen”, and even its 3:1 F2 segregation. The various colors are thus determined by different genes.
The relationship between yellow-grained F2 plants and resistance to SBCMV found in this study is at least worth mentioning (Fig. 7). While Rümker and Leidner (1914) observed a monogenic dominant inheritance from green (dominant) to yellow (recessive) seed color in rye, later, Sturm et al. (1981) localized the gene for green color seed (An1) on chromosome 2R (Schlegel 2020).
Thus, the recessive allele for the seed color on chromosome 2R (an1) could be related to the locus for resistance to SBCMV. Further investigations are initiated in order to clarify this linkage.
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Schlegel, R., Eifler, J., Schmidt, M. et al. Screening and genetic studies on resistance to Soil-born Cereal Mosaic Virus (SBWMV) in rye. CEREAL RESEARCH COMMUNICATIONS 49, 401–412 (2021). https://doi.org/10.1007/s42976-020-00105-1
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DOI: https://doi.org/10.1007/s42976-020-00105-1