Resistance to biotic and abiotic stress in potato: the origin of the genes and corresponding molecular markers

The integration of molecular markers in the realm of potato genetics has opened new avenues for accelerating genotype analysis and developing improved varieties. Many markers linked to important features have been discovered so far and are consistently distributed across 12 chromosomes (× = 12) of potato. Notably, the genes allied to disease resistance stand out as significant and prevalent. Molecular markers associated with these genes have revolutionized selection processes, making them faster and more effective. Besides, advanced technologies such as kompetitive allele-specific PCR, high-resolution melting assay, SNP-array, genotyping by sequencing, and genome-wide association study, are emphasizing the use of those molecular markers with greater accuracy to detect R genes aligning with the phenotypes. This review discusses advances in potato breeding for resistance against common stresses, focusing on progress made through molecular marker-assisted selection.

Potato, Solanum tuberosum L, is an associate of the Solanaceae family and one of the world’s top four widely grown crops. The appeal of potatoes lies in their nutritious content and high production rate per unit of time and area, making them particularly valuable in underdeveloped nations (Islam et al. 2022). Apart from being a staple food, potatoes are widely utilized in various industries for the production of a diverse range of products. Furthermore, its vast range of applications, including food, alcohol, starch-based products, and raw materials, have made it quite popular in industrialized countries (Awasthi and Verma 2017). Owing to the vital importance of potato, it is imperative to enhance potato production. Its yield potential, on the other hand, is often reduced due to its high susceptibility to numerous disease invasions including various soil-borne pathogens and viruses (Awasthi and Verma 2017; Chakrabarti et al. 2022). Such infestations increase the use of fungicides or insecticides for disease management which reduces the grower’s profit margins (Islam et al. 2018). In addition to biotic pressures, abiotic factors, such as drought, low temperature, and salinity, have caused challenges for producers during potato cultivation (Kikuchi et al. 2015). Therefore, both biotic and abiotic factors play major roles as stressors for potato cultivation. Subsequently, identifying molecular markers that are used to screen potatoes for resistance to these stresses, can be a remedy to overcome those stresses (Mangal et al. 2023).

However, among the various stresses, late blight (LB), caused by Phytophthora infestans, is one of the most prevalent and disruptive diseases that affect potato cultivation worldwide (Islam et al. 2022). In the severely affected potato field, LB can cause deprivation of yield by 70–100% (Islam et al. 2018). In order to lessen the impact of the disease, a significant amount of fungicides was applied, which resulted in increasing the cost of 6.7 billion USD using fungicides for growers (Seidl Johnson et al. 2015). Moreover, potato viruses, such as potato virus Y (PVY), potato leaf roll virus (PLRV), potato virus M (PVM), potato virus S (PVS), potato virus X (PVX), and potato virus A (PVA), are other disease-causing agents that have also a significant impact on yield. Hence, minimizing the risks in potato production by viruses is justifiably a crucial concern in the breeding of potatoes (Bhardwaj et al. 2019; Slater et al. 2020; Kumar et al. 2022). Furthermore, potato cyst nematodes (PCN) caused by Globodera rostochiensis and Globodera pallida (Price et al. 2021), and root-knot nematodes caused by Meloidogyne sp. (Khan et al. 2023), affect the growth rate and physiology of potatoes, respectively, resulting in weight loss. However, to reduce the disease impact of nematodes, farmers usually apply granular nematicides (Grabau and Noling 2019) which cost a lot of money.

Like biotic stressors, potato is also more vulnerable to abiotic stressors than other plants. It is anticipated that, by the year 2050, the anticipated reduction in overall potato yield may potentially reach as high as 32% as a consequence of the influence of abiotic stress factors (Demirel 2023). Drought and salinity tolerance are said to be extremely low in potatoes (Kikuchi et al. 2015) due to their inability to acclimate to low temperatures and potato seedlings stop growing below 7 °C and experience chilling, frost, and death below −0.8 °C, −2 °C, and −3 °C, respectively (Yan et al. 2021). Besides, the rising temperatures and environmental pressures threaten the existence of wild potato relatives, which are crucial gene pools for breeding new potato varieties adapted to abiotic stress (Hussain 2016). In light of the aforementioned challenges, it is imperative for plant breeders to focus their efforts on developing crop varieties resistant to both biotic and abiotic stresses. The convergence of pathogens and climate change presents a dual challenge to crop cultivation, constraining yields through a combination of biotic and abiotic stresses (Haq et al. 2022).

Field evaluation and phenotypic screening in traditional breeding can span 10–15 years due to the need for multi-generational backcrossing (Tiwari et al. 2013). On the other hand, employing genotype analysis using a molecular marker to detect and select suitable species with desired traits has grown increasingly popular day by day (Caruana et al. 2019). This selection approach is known as marker-assisted selection (MAS). MAS uses a significantly cheap selection strategy per cultivar in potato breeding compared to traditional phenotypic screening in the field (Slater et al. 2020). MAS identifies molecular markers, which corresponds to genes displaying the desired trait, from the genome of a particular species (Simko et al. 2013). It is also more reliable and precise since this method is independent of environmental conditions. Furthermore, the genetic map of potatoes is an integral part of the identification of molecular markers that are connected to the desired trait such as resistance to a certain disease (Caruana et al. 2019). Molecular markers can also be designed to identify quantitative trait loci (QTL), which are genetic loci responsible for controlling specific quantitative traits such as yield and tuber quality (Habe et al. 2019; Fenstemaker et al. 2023).

Hence, molecular markers can be used along with traditional breeding technology to pinpoint the exact genotype that expresses the desired attribute, such as disease resistance (Fig. 1). An informative marker has a strong relationship between the phenotypic trait and the gene and is close to the specific locus. Markers, such as simple sequence repeats (SSR), restriction fragment length polymorphism (RFLP), amplified fragment length polymorphism (AFLP), sequence characterized amplified regions (SCAR), and cleaved amplified polymorphic sequence (CAPS), are the well-known molecular markers currently utilized in potato breeding (Kumar and Jorben et al. 2023). Furthermore, high-resolution melting analysis (HRM) is a relatively new technology that distinguishes amplicons of alleles with different haplotypes (one or more SNPs) (Nie et al. 2016; Meiyalaghan et al. 2018). HRM could detect homozygosity of morphological and genetic features in a single genetic map and identify resistant genes against numerous diseases (Nie et al. 2018).

Harnessing the potato gene pools for enhanced resistance to biotic and abiotic stresses in new cultivars

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However, it is critical to identify the exact disease-resistance gene using gene-specific markers. Several researches have been undertaken on different potato virus-resistant gene markers, including PVY (Bhardwaj et al. 2019; Slater et al. 2020), PLRV (Mihovilovich et al. 2014; Yermishin et al. 2016), and PVX (Fuentes et al. 2021; Liu et al. 2021). Additionally, a large number of researchers have generated LB-resistant potato varieties where the resistance genes’ sources were taken mostly from potato wild-type varieties, S. demissum (6×), S. berthaultii (2×), and S. Stoloniferum (4×) (Tiwari et al. 2013; Ramakrishnan et al. 2015). Such resistant genes against LB include R1 (Ballvora et al. 2002; Khavkin et al. 2010; Rogozina et al. 2021), R2 (Lokossou et al. 2009; Sokolova et al. 2014; Rogozina et al. 2021), R3 (a/b) (El-Kharbotly et al. 1996; Tiwari et al. 2013; Rogozina et al. 2021), Rpi-smira 1 & 2 (Jo et al. 2011; Tomczynska et al. 2014), Rpi-bt1 (Oosumi et al. 2009; Ramakrishnan et al. 2015), Rpi-blb1 (Naess et al. 2000; Tiwari et al. 2013), Rpi-ber (Park et al. 2009; Islam et al. 2018),and so on. Similarly, different resistant genes against potato cyst nematodes have also been reported including H1 (Ellenby 1952; Asano et al. 2012; Chekushkina et al. 2020), H2 (Strachan et al. 2019), H3 (Bradshaw et al. 1998), GroV1 (Jacobs et al. 1996), Gro1 (Barone et al. 1990), and Gpa2 (Asano et al. 2012).

Thir review focuses on addressing abiotic and biotic stress factors affecting potato cultivars. The main objective is to provide insights into resistance genes, their sources, and associated markers that can aid in identifying potato species resistant to common diseases and key abiotic factors. By doing so, it aims to expedite the cultivar selection process, enabling more efficient breeding prograns and advancements in potato breeding.

Virus resistance genes and linked markers

Viral infections can be detrimental to crop production, resulting in reduced yields as the severity of the disease increases (Tiwari et al. 2022). There are approximately 50 viruses that can infect Solanum at various stages of growth and among them, six potato viruses are the most prominent due to their devastating yield impact (Kreuze et al. 2020). PVY is identified to be the deadliest virus for potatoes as it can decrease the yield from 30 to 80%. PLRV, the second most destructive disease, can reduce yield loss by up to 20 million tonnes per year (Kreuze et al. 2020). On the other hand, the disease symptoms appear to increase in severity depending on certain combinations of viruses; such as the combinations between the PVY, PVS, PVX, PVM, and PVA (Kreuze et al. 2020).

As a result, constant efforts were carried out to introduce resistance genes into commercial potatoes to lessen the harm (Ramakrishnan et al. 2015). Virus-resistance genes have been found in a variety of wild potato species. Extreme resistance genes for PVY have been isolated from S. Stoloniferum (4X) or S. tuberosum ssp. andigena (2X) (Hamalainen et al. 1998; Ramakrishnan et al. 2015). R genes, Ry_adg and Ry_sto, have been shown to exhibit resistance against PVY (Table 1), localized on chromosomes XI and XII (Fig. 2), are from S. tuberosum ssp. andigena (2×) and S. stoloniferum (4×), respectively (Ramakrishnan et al. 2015; Yermishin et al. 2016). Moreover, R genes, Ny_tbr and Ry_chc, are located on chromosomes IV and IX, from S. berthaultii (2X) and S. Chacoense (2X), respectively (Table 2) (Park et al. 2005; Ramakrishnan et al. 2015). Hence, various molecular markers linked to such R genes have been developed to identify resistant potato varieties (Ramakrishnan et al. 2015). For instance, markers SC895 and TG506 are connected with N-genes, Ny_-1 and Ny_tbr, known to exhibit hypersensitivity to the potato virus Y ( Additional file 1: Table S1). On the other hand, markers RYSC3 (Sharma et al. 2014; Kneib et al. 2017; Bhardwaj et al. 2019; Slater et al. 2020), M45 (Kneib et al. 2017; Bhardwaj et al. 2019; Slater et al. 2020), ADG1, and ADG2 (Hamalainen et al. 1998) are associated with the R gene Ry_adg; GP122 (Valkonen et al. 2008; Lopez-Pardo et al. 2013), STO4 (Cernak et al. 2008), Yes3-3A (Song and Schwarzfischer 2008; Bhardwaj et al. 2019), and Yes3-3B (Song and Schwarzfischer 2008) are linked with the R gene Ry_sto; and markers RY186 (Kneib et al. 2017; Rogozina et al. 2019; Biryukova et al. 2020), CT220 (Rouppe Van der Voort et al. 2000), and TG506 (Park et al. 2005) are associated with the R gene Ry_chc (Table 1 and Additional file 1). These R genes have been demonstrated to be extreme resistance to PVY.

Mapping genomic locations of biotic and abiotic stress resistance genes in potato on the 12 chromosomes

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Additionally, PVX resistance genes have been bred into S. tuberosum (4×) from S. tuberosum ssp. andigena (2×) mostly (Mori et al. 2011; Yermishin et al. 2016; Bhardwaj et al. 2019) and in some cases from S. demissum (6X) (Marano et al. 2002). The majority of N- genes markers are CAPS markers, where the Ny_-1 and Ny_tbr confer hypersensitivity towards PVY, whereas Nb-genes exhibit PVX resistance (De Jong et al. 1997; Szajko et al. 2014). In addition, the Nc_tbr gene and a new putative gene Nz_tbr were also reported to confer hypersensitive resistance against PVY (Table 2) (Chik-Ali 2014). Furthermore, resistance genes for PVS were also bred from S. tuberosum ssp. andigena and Ns gene-affiliated markers SC811, CP16, and SCG17-321 revealed extreme resistance against PVS (De Jong et al. 1997; Bhardwaj et al. 2019). Moreover, the resistance for PVX is determined by Rx genes, that is Rx1 and Rx2, which are localized on chromosomes XII and V, respectively (Table 2) (De Jong et al. 1997; Nie et al. 2016, 2018). Nevertheless, research to date shows the resistance genes for PLRV are constituted in clusters of the PLRV.1 (Table 1) and PLRV.4 genes from chromosome XI, and PLRV.2 and PLRV.3 in chromosomes VI and V, respectively or the Rladg gene from chromosome V (Marczewski et al. 2004).

Late blight-resistant genes and linked markers

P. infestans causes rapid mutation against the plant’s defense mechanism leading to the most destructive disease known as potato late blight (LB), so it has been the subject of ongoing and intense research for over a century (Ramakrishnan et al. 2015; Ivanov et al. 2021). To produce LB-resistant varieties, genes conferring resistance to LB were introduced from various wild potato varieties and cultivated species. As the LB-resistant genes are linked to R genes, a screening method utilizing R gene-associated markers was proposed to identify LB-resistant potato species (Ramakrishnan et al. 2015).

Resistant gene R1 has been discovered in S. demissum (6×) (Ballvora et al. 2002; Bormann et al. 2004; Bhardwaj et al. 2019; Rogozina et al. 2021), S. berthaultii (2×), S. hjertingii (4×), S. stoloniferum (4×), and S. pinnatisectum (2×) (Sokolova et al. 2014) (Table 2). This R1 gene can be detected with the markers CosA (Sharma et al. 2014; Bhardwaj et al. 2019), R1 (Bhardwaj et al. 2019), R1-1205 (Sokolova et al. 2014), BA47f2 (Tiwari et al. 2013), GP76 (Oberhagemann et al. 1999), GP179 (Tiwari et al. 2013), and GP 21 (De Jong et al. 1997; Tiwari et al. 2013) (Table 1 and Additional file 1: Table S1). The R1 gene localized in chromosome V (Fig. 2) of S. demissum (6×) was even introgressed in the cultivated species S. tuberosum (Ballvora et al. 2002; Ramakrishnan et al. 2015; Rogozina et al. 2021). Apart from R1, several other significant R genes found in S. demissum (6×) are R2, R3a, and R3b (El-Kharbotly et al. 1996; Lokossou et al. 2009; Sokolova et al. 2014; Rogozina et al. 2021). Resistant gene R2 can be targeted through SSR marker R2 (Kim et al. 2012); R3a gene can be targeted by markers R3 (Bhardwaj et al. 2019) and R3a (Sokolova et al. 2014); R3b gene can be identified through the marker R3b (Sokolova et al. 2014). Tiwari et al. (2013) also mentioned that R3 genes (both R3a and R3b) residing on chromosome XI can be screened through R3-1380 (Sokolova et al. 2014), SHa (Huang et al. 2005), and R3b4 (Rietman 2011) markers. Other common sources for R2, R3a, and R3b genes can be S. bulbocastanum (2×), and S. hougasii (6×) (Table 2) (Sokolova et al. 2014; Sharma et al. 2014; Bhardwaj et al. 2019). Additionally, other LB-resistant R genes such as Rpi-blb1 can be targeted either by SCAR markers like Rb-1223 (Tiwari et al. 2013) and RB-629/638 (Sokolova et al. 2014; Tiwari et al. 2013) or SSR markers such as BLB1 (Chen et al. 2017) and 1521/518 (Additional file 1: Table S1) (Tan et al. 2010; Islam et al. 2022) found in S. bulbocastanum (2×), S. hjertingii (4×), S. berthaultii (2×), and S. stoloniferum (4×) (Table 2) (Sokolova et al. 2014). Again, 45/XI can target the resistance gene Rpi-Smira1, located in the same region as the gene R3 of Chromosome XI in S. phureja (2×) (Tomczynska et al. 2014; Islam et al. 2022). Rpi_-Smira2, a different Rpi gene traced on chromosome IX (Fig. 2) was undergoing field trial (Jo et al. 2011; Tomczynska et al. 2014). The rest of the Rpi genes, Rpi_-bt1 and Rpi_-ber (Table 1), were found scattered and constituting in different chromosomes such as chromosomes VIII and X (Fig. 2) (Tiwari et al. 2013; Ramakrishnan et al. 2015; Islam et al. 2022).

Potato cyst nematode-resistant genes and linked markers

Potato cyst nematode (PCN) is a soil-borne disease caused by golden nematode which has long been recognized in Europe as a serious potato pest that reduces total potato yield. An efficient solution to produce PCN-free potatoes is to incorporate PCN-resistant genes in the cultivars. Numerous PCN-resistant genes have been identified with varying degrees of resistance, genes Gro1.4, Gpa, Gpa4, Gpa5, Gpa6, Grp1, Gro1.2, and Gro1.3 were found with limited resistance to PCN, whereas H1 (Ellenby 1952), Gro1 (Barone et al. 1990), GroV1, and Gpa2 (Asano et al. 2012) genes (Table 1) express strong resistance. Many of these genes are condensed in a precise location, including the QTL, consisting of Grp1, Gpa3, Gpa5, and Gpa6. H1, a heterozygous dominant gene obtained from S. tuberosum ssp. andigena (2×) located on chromosome V has been valuable commercially for decades for its resistant durability to the Globodera rostochiensis (Gartner et al. 2021). The CP113 marker, which was created during ultra-high-density genetic mapping of the H1 locus (Bakker et al. 2004), was found to be one of the most closely linked markers to the H1 gene, while other markers such as GP22, GP265, GP270, GP78, and GP188, which are close in distance to CP113, were also linked to the H1 locus (Gebhardt et al. 2006). Besides, the markers, 239E4left, CT51 (Bakker et al. 2004), N146, N195 (Asano et al. 2012), were also found to be linked with the PCN extreme resistance gene H1 (Table 1 and Additional file 1: Table S1). Again, Gro1 was the first highly dominant G. rostochiensis resistant gene, located on Chromosomes VII and IX (Fig. 2), and was mapped with RFLP markers (Barone et al. 1990; Barone et al. 2004). Moreover, the H2 nematode resistance gene was mapped to chromosome V’s distal end in tetraploid potato (Strachan et al. 2019).

Other potato disease-resistant genes and linked markers

Markers can help to screen for many other potato diseases, such as potato warts, potato blackleg, potato scab, and potato wilt. The PCR-based marker N125, which is designed to target the resistance gene Sen1 (S. endobioticum pathotype 1), located at a position on chromosome XI similar to Ryadg genes, can be used to screen for potato wart resistance (Gebhardt et al. 2006). While the AFLP markers can be used to test resistance against potato blackleg disease through the blackleg disease-resistant gene Eca, mapped to all 12 potato chromosomes (Zimnoch‐Guzowska et al. 2000). Moreover, researchers have successfully identified a few genes conferring resistance to Streptomyces, the causative agent for the common scab. Some resistant genes were reported to have been isolated from chromosome XI of the S. chacoense (2×) (Kaiser et al. 2020). Previously, a study conducted by Flores et al. reported having accomplished to design of Stx1a and Stx1b markers for txtA and txtB genes mapped from S. acidiscabies (Flores‐González et al. 2008). Furthermore, 4 PCR-based primer pairs, namely ScabI and ScabII, TurgI and TurgII, AurI andAurII, pA and pH' have been developed for genes that confer resistance to S. turgidiscabies and S. scabies in potato species S. tuberosum (Lehtonen et al. 2004). The resistance genes qBWR-2, qBWR-3, and qBWR-4, which protect potatoes from bacterial wilt (BW) caused by Ralstonia solanacearum, were found in potato chromosomes III, VII, and X, respectively (Habe et al. 2019). To find the BW-resistant genes in potatoes, researchers used a variety of markers, including RAPD, SSR, and AFLP. SSR marker STM0032 on chromosome XII and three RAPD markers, OPG05₉₄₀, OPR11₈₀₀, and OPO13₇₇₀, were discovered to be tightly connected to the bacterial wilt-resistant gene in potatoes (Patil et al. 2012). Additionally, the suppression subtractive hybridization and microarray techniques were applied by Li et al. (2010) to identify genes that confer resistance to R. solanacearum in potato and STA51, STC84, and STD62, as well as STSN2 (STM21), had been identified as significant resistance genes to BW. Besides, expression of the genes snakin1 and snakin2 genes in potato were also found to boost BW resistance (Li et al. 2010). Alternatively, over-expression of these two genes Snakin-1 and Snakin-2 encoded the proteins Gibberellin Stimulated-Like 1 (Jacobs et al. 2022) and Gibberellin Stimulated-Like 2 (Mohan et al. 2014), respectively, in transgenic potato, were also conferred resistance to blackleg disease caused by Pectobacterium atrosepticum. In addition, early blight, caused by Alternaria solani, is also one of the major diseases in potato worldwide, and up to 54% yield loss occurs without fungicide application (Abuley et al. 2018; Xue et al. 2022). The early blight resistance in potato is highly heritable, with high broad sense and narrow sense heritability. Two wild potato species, S. berthaultii and S. commersonii subsp. malmeanum, exhibits promising resistance against early blight (Wolters et al. 2021). Genetic mapping-identified QTLs on chromosomes V and VII contribute to early blight resistance, providing potential markers for breeding resistant varieties (Xue et al. 2022). Although earlier studies had limitations such as small population sizes and incomplete linkage maps, the development of high-density SNP marker linkage maps has made QTL mapping more convenient in potato research (Odilbekov et al. 2020). Further research is needed to determine more accurate genetic basis resistance to early blight.

In addition to the aforementioned diseases, the potato confronts a spectrum of other significant maladies that exert substantial economic and agricultural impact. These afflictions include pink rot (Phytophthora erythroseptica), pythium leak (Pythium ultimum), dry rot (Fusarium oxysporum), soft rot (Dickeya dianthicola, Pectobacterium spp.), silver scurf (Helminthosporium solani), and black dot (Colletotrichum coccodes). These phytopathogens manifest their detrimental influence predominantly during the storage phase of potatoes. Hence, Osusky et al. (2004) found that MsrA3, a modified form of the naturally occurring antimicrobial cationic peptide temporin A, when expressed in potato plants, conveys strong resistance to late blight and pink rot. On the other hand, Thompson et al. (2007) reported that a potato clone derived from S. berthaultii and S. etuberosum exhibited resistance to P. erythroseptica and P. ultimum. Besides, the inheritance of dry rot resistance was investigated by Sobkowiak et al. (2022) in two diploid potato hybrid populations, leading to the identification of multiple QTLs on chromosomes II, VII, IX, and XII, including the first mapping of loci affecting tuber dry rot resistance in the potato genome. However, the dry rot resistance genes might derived from the wild-type potato S. chacoense, S. microdontum, and S. gourlayi as they were shown extreme resistance to dry rot (Sobkowiak et al. 2022). Moreover, consistent QTLs for soft rot resistance from wild potato S. microdontum were spotted in chromosomes I, III, and V, responsible for resistance to Dickeya dianthicola (Fenstemaker et al. 2023). Henceforth, increasing more extensive research activities on those diseases will help in understanding the molecular underpinnings of resistance mechanisms against these diverse pathogens which is pivotal for the development of improved potato cultivars with enhanced storage durability.

Drought tolerance genes and linked markers

A deficit in the water supply may adversely affect various developmental stages of potatoes, especially limiting their growth, reproduction, tuber quality, tuber size, and yield (Anithakumari et al. 2011). Numerous genes involved in carbohydrate metabolism, cellular communication, protein synthesis, ATP metabolism, and cell signaling are upregulated or downregulated when exposed to water stress (Ambrosone et al. 2011). The expressions of such genes have been evaluated within potato tissues under drought conditions and adequate water conditions (Obidiegwu et al. 1999). Using SNP markers revealed 23 QTLs related to drought tolerance phenotypes (Anithakumari et al. 2011). Moreover, five specific genes, ACS3, ALDH, ETRTF3, PARG, and PP2C, encoding 1-aminocyclopropane-1-carboxylate synthase 3, aldehyde dehydrogenase, ethylene-responsive transcription factor, poly (ADP-ribose) glycohydrolase, and protein phosphatase 2C, respectively, have been reported being present in drought-sensitive cultivars. These ACS3, ALDH, ETRTF3, PARG, and PP2C genes were discovered on potato chromosomes I, II, IV, X, and XII using SSR markers HRO_ACS3_1, HRO_ALDH_H, HRO_ETRTF_5a_D, HRO_PARGH_1A_B, and HRO_PP2C_1_B, respectively (Table 3) (Ghislain et al. 2009; Schumacher et al. 2021). Furthermore, the positions of these genes associated with drought resistance are not fixed to one specific allele rather the locations vary in alleles among different potato varieties, making them ideal candidates for MAS as well as genetic diversity analysis (Malosetti et al. 2007). Moreover, the presence of an extra allele in drought-sensitive cultivars suggests that the selection of cultivars against these alleles will facilitate the selection of drought-tolerant varieties (Schumacher et al. 2021).

Cold tolerance genes and linked markers

The potato is a highland crop that grows in cold regions, yet frost damage in cold climates is also a significant issue in potato production. Cold stress stunts potato growth and development, resulting in lower yields (Tu et al. 2021). Even though there are some wild potato species with cold tolerance characteristics yet a commercial cultivar with such characteristics is yet to be found. In terms of cold tolerance, S. commersonii (2×/3×) showed supreme tolerance against cold and was potent to resist frost and achieved tuber hardening in a temperature range from 2 to 12°C. Furthermore, S. acaule (4×) showed remarkable resistance to cold stress whereas S. tuberosum (4×), S. verrucosum (2×/3×/4×), and S. stoloniferum (4×) showed the most sensitivity to cold stress (Kikuchi et al. 2015; Ramakrishnan et al. 2015). Besides, it was reported that S. tuberosum hybrids had been made with S. brevidens and S. commersonii (2×/3×) to get a cold stress-resistant breed (Orczyk et al. 2003). Tu et al. (2021) conducted a study on the hybridization of S. malmeanum (2×/3×), a wild species known for its strong freezing tolerance, with the freeze-sensitive commercial cultivar S. tuberosum, with the goal of creating improved varieties that are more tolerant to freezing. And after hybridization via protoplast fusion, the somatic hybrids were screened with eight SSR primers, S215, ssr_165426, ssr_165497, ssr_165552, ssr_165648, ssr_165659, S165, and ssr_166097. On the other hand, some heat shock transcription factors (HSTF), StHsf004, StHsf007, StHsf009, StHsf014, StHsf018, StHsf019, and StHsf022 genes were found with potentiality against cold stress (Table 3 and Fig. 2). Previously, the roles of HSTFs were confirmed for cold stress via RT-qPCR using specific markers named by their corresponding gene names (Tang et al. 2016).

Further research on technological advancements, and high throughput technologies are being practiced for unlocking the full potential of molecular markers in developing improved disease-resistant potato (Fig. 3). High throughput genotyping technologies such as genotyping by sequencing (GBS) was applied to discover dense markers for detecting disease resistance and other important traits in potato and a significant number of SNP markers were identified and filtered to create a high-quality subset (Caruana et al. 2019). In addition, high throughput melting (HRM) assay was employed to detect H1-linked resistance to potato cyst nematode. The HRM assay utilized the markers TG689 and 57R-1P for this purpose (Meiyalaghan et al. 2018). In another study by Nie et al. (2018), the markers 5Rx1 and 106Rx2 were utilized in HRM to identify the PVX resistance genes Rx1 and Rx2, respectively. Nie et al. (2016) employed the YES3-3A marker in an HRM assay to precisely locate the PVY resistance gene Rysto in potato (Table 4). However, another high throughput genotyping technology, namely kompetitive allele-specific PCR (KASP), is a rapidly emerging high throughput genotyping technology, particularly popular for single nucleotide polymorphism (SNP) based analyses. It is a homogeneous and fluorescence-based genotyping variant of the PCR method. In the realm of potato genotyping, numerous studies have already reported the successful application of KASP. For instance, Sood et al. (2022), Kante et al. (2021), and Caruana et al. (2021) have utilized KASP to confirm the presence of resistance genes Ry_adg and Ry_sto against potato virus Y, employing the marker M6 and YES3-3A, respectively (Table 4). Additionally, KASP has proven valuable in identifying various late blight resistance genes, including Rpi_-cap1 (Ram et al. 2018), R2 (Meade et al. 2020), Rpi_-blb3 (Karki et al. 2021), R8 (Sood et al. 2022), and RB/Rpi_-blb1 (Sorensen et al. 2023), across different late blight-resistant genotypes. Furthermore, KASP technology has been effectively employed to detect potato cyst nematode resistance genes H1, using the marker 57R (Meade et al. 2020) and H2, through the markers CPRISNP 01–11 (Sood et al. 2022). Indeed, the SNP array is another powerful SNP-based genotyping technology that has been effectively utilized in potato genotyping, particularly in the detection of resistance genotypes. Prodhomme et al. (2020) employed the SNP array to identify specific markers, namely hs-SNP, STM1002-24, and St1004-96, associated with the potato wart disease resistance genes Sen1 (Prodhomme et al. 2020), Rse-Ivb, and Rse-VIa (Obidiegwu et al. 2015), respectively. Moreover, the SNP array has also been instrumental in detecting the marker MG-64-17, which is associated with the PVY resistance gene Ry_chc (Table 4), as demonstrated by Li et al. (2022). Nonetheless, genome-wide association studies (GWAS) have been conducted to identify the genomic regions associated with resistance in potato such as GWAS was employed to locate genetic markers linked to resistance against late blight (Prakash et al. 2020; Wang et al. 2020) and potato common scab (Yuan et al. 2020).

A schematic for high-throughput genotyping in potato breeding using conventional primers connected to genes for disease resistance

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On the other hand, the current understanding of genotyping technologies for detecting abiotic stress tolerance genes in potato is relatively limited. However, Anithakumari et al. (2011) made significant strides in this field by identifying several SNP-based markers associated with drought stress in potatoes. Notably, they observed that the gene markers PotSNPs (PotSNP838, PotSNP67) were co-located with the root-to-shoot ratio QTL, suggesting a potential link between these markers and improved drought tolerance in potatoes. Since plants with an increased root-to-shoot ratio are reliable indicators of drought adaptation. Besides, researchers demonstrated proactive efforts in a separate study by transferring the AtDREB1A gene from Arabidopsis thaliana to tetraploid potatoes. This gene was found to function as a transcriptional factor, imparting enhanced protection against various abiotic stresses, particularly drought and salt (Watanabe et al. 2011). These findings underscore the potential of genetic engineering to enhance abiotic stress tolerance in potato crops. Moving forward, addressing the challenges in this area will necessitate a more comprehensive exploration of potato genetic resources with altered functions related to abiotic stress tolerance, particularly those sourced from wild potato species. Fundamental research efforts should focus on elucidating the molecular mechanisms and physiological functions of these tolerances, which will inform the development of effective germplasm enhancement strategies using genetic resources. Moreover, parallel efforts should be directed towards harnessing exotic genes to augment the potato's capacity to withstand extreme abiotic stresses. Such scientific endeavors hold great promise for the advancement of resilient potato varieties, better equipped to thrive under challenging environmental conditions.

Even in tetraploid plants such as potatoes, molecular markers help to transport valuable genes and allow for the selection of superior genotypes. Potato disease resistance molecular markers have revolutionized the field of agriculture by offering advanced tools for breeding and potato improvement programs. However, resistance genes for late blight (R1, R2, R3a, R3b, and Rpi-genes), PVY (Ry_adg, Ry_sto, and Ry_chc), PLRV (PLRV1), PVX (Rx1 and Rx2), PVS (Ns), and PCN (H1, H2, Gpa2, Gor1-4, and Gpr1) are available in potato and these R genes linked molecular markers are widely used in potato breeding for the genetic gain against those destructive diseases (Asano et al. 2012; Yermishin et al. 2016; Kneib et al. 2017; Bhardwaj et al. 2019; Klimenko et al. 2019; Chekushkina et al. 2020; Slater et al. 2020).

The benefits of molecular markers for enhancing potato disease resistance are multifaceted. They offer remarkable speed and precision in the breeding process, allowing for the early identification of disease-resistant plants. For instance, Sharma et al. (2014) successfully employed molecular markers to identify elite germplasm with resistance to late blight (R1, R2, and R3a), potato virus Y (Ry_adg and Ry_sto), and potato cyst nematode (H1 and Gro1-4). Besides, marker-assisted selection (MAS) facilitates the introduction of resistance genes into elite cultivars without compromising desirable traits, while simultaneously decreasing breeding costs and time requirements, as reported by Bhardwaj et al. (2019) for resistance to potato viruses (PVY, PVS, PVX, and PLRV). Moreover, molecular markers enable the pyramiding of multiple resistance genes, as demonstrated by Mori et al. (2011) in their development of a multiplex PCR to spot resistance genes for late blight, PVX, PVY, and PCN. Similarly, another multiplex PCR protocol was developed by Rogozina et al. (2019) to identify potato genotypes for breeding R genes resistance to PVY (Ry_sto, Ry_chc), PVX (Rx), PCN (H1 and Gro1-4), and potato wart (Sen1) disease. This broadens genetic diversity and bolsters resistance against various diseases. They also aid in the conservation of genetic diversity by preserving rare and unique disease-resistant genes in wild relatives, ensuring the long-term sustainability of potato production in the face of evolving disease pressures.

However, potato breeding for disease resistance using molecular markers faces significant challenges in practical implementation. The diverse and complex nature of potato diseases, combined with the indirect link between molecular markers and resistance genes, leads to potential false results. Moreover, the tetraploid nature of potatoes makes it difficult to identify and track genes, which further affects the accuracy of marker-based breeding. Addressing the challenges, several advanced genotyping technologies have already been established such as genotyping by sequencing (GBS), high-resolution melting (HRM), kompetitive allele-specific PCR (KASP), SNP array, genome-wide association studies (GWAS), and so on. Those technologies offer several advantages for potato breeding in terms of disease resistance. They are (a) highly precise, reducing errors, and enhancing the accuracy of genetic variation detection; (b) more sensitive in identifying disease-associated genetic variations; (c) possess superior resolution, enabling the detection of subtle genetic variations linked to resistance genes; (d) high-throughput, allowing for the simultaneous identification of multiple resistance genes; (e) capable of detecting numerous single nucleotide polymorphisms (SNPs) across the genome, facilitating a comprehensive analysis of genetic diversity and the discovery of new resistance genes; (f) cost-effective and efficient, facilitating the selection of disease-resistant potato varieties. Moreover, the unlabeled probe HRM assay has the capability to detect allele dosage, which can be considered an additional advantage of advanced genotyping technologies (Meiyalaghan et al. 2019).

Finally, it might be concluded that based on the molecular markers’ researchers can perform high-throughput technology like SNP-depended technologies, KASP, HRM, target SNP-seq as well as develop new technologies to identify more efficient and specific resistance gene locus for genotyping the potato breeding population against different biotic and abiotic stresses.

Raw sequence data of the resistance genes are available in the NCBI (https://www.ncbi.nlm.nih.gov/) portal and the chromosomal location of the resistance genes is retrieved from Spud (http://spuddb.uga.edu/). Besides the information markers linked to R genes are listed in the supplementary documents attached to this manuscript as Additional file 1.

ACS3:

1-Aminocyclopropane-1-carboxylate synthase 3

AFLP:

Amplified fragment length polymorphism

ALDH:

Aldehyde dehydrogenase

BW:

Bacterial wilt

CAPS:

Cleaved amplified polymorphic sequence

ETRTF3:

Ethylene-responsive transcription factor

GBS:

Genotyping by sequencing

GWAS:

Genome-wide association study

HRM:

High-resolution melting

KASP:

Kompetative allele-specific PCR

LB:

Late blight

MAS:

Marker-assisted selection

PARG:

Poly (ADP-ribose) glycohydrolase

PCN:

Potato cyst nematode

PCR:

Polymerase chain reaction

PLRV:

Potato leaf roll virus

PP2C:

Protein phosphatase 2C

PVA:

Potato virus A

PVM:

Potato virus M

PVX:

Potato virus X

PVY:

Potato virus Y

QTL:

Quantitative trait loci

RAPD:

Random amplified polymorphic DNA

RFLP:

Restriction fragment length polymorphism

SCAR:

Sequence characterized amplified regions

SNP:

Single nucleotide polymorphism

SSR:

Simple sequence repeats

StHsf:

Heat shock transcription factor

The authors gratefully acknowledge Dr. Jianke Dong for assisting in the bioinformatics analysis. We also thank the editors and reviewers who dedicated their time, expertise, and insights to improve this work.

This work was supported by the National Natural Science Foundation of China (31971989) and the China Agriculture Research System of MOF and MARA (CARS-09-P07).

Authors and Affiliations

1. Key Laboratory of Potato Biology and Biotechnology (HZAU), Ministry of Agriculture and Rural Affairs, National Key Laboratory for Germplasm Innovation and Utilization of Horticultural Crops, Huazhong Agricultural University, Wuhan, 430070, China

   Saiful Islam, Jiana Li, Fangru Xie, Botao Song & Bihua Nie

2. Advanced Seed Research and Biotech Centre, ACI Limited, Gulshan Avenue, Dhaka, 1212, Bangladesh

   Mohammad Ataur Rahman

Contributions

S.I. collected the gene information from online portals such as NCBI or Ensemble Plants, wrote the original draft, and helped in final editing, L.J. performed to review and corrections, M.A.R. performed the literature collection and helped with the writing of the original draft, X.F. performed literature review, B.S. performed review, final editing, and corrections, B.N. performed conceptualization, final review, and editing, corrections.

Corresponding author

Correspondence to Bihua Nie.

Ethics approval and consent to participate

Not applicable.

Consent for publication

Not applicable.

Competing interests

The authors declare that they have no known competing interests that could have appeared to influence the work reported in this paper.

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