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Marker assisted back cross

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Guruprasad SA

Introduction Backcross breeding & its types Marker assisted breeding Marker assisted backcross breeding (MABC) Main strategies Advantages over conventional breeding Case studies Future outlook Conclusion

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Marker Assisted Backcross Breeding (MABC) in Crop Improvement
●Introduction ●Backcross breeding & its types ●Marker assisted breeding ●Marker assisted backcross breeding (MABC) ●Main strategies ●Advantages over conventional breeding ●Case studies ●Future outlook ●Conclusion Flow of seminar
● Backcross breeding is a well-known procedure for the introgression of a target gene f ● The objective is to reduce the donor genome content (DGC) of the progenies by repe Backcrossing 6
Factors necessary for backcross method: (i) Recurrent parent Selection (ii) Screening for target trait (iii) Number of backcrosses ●To transfer a major gene ● In disease/pest resistance breeding ● To transfer alien cytoplasm or to transfer cytoplasmic male sterility ●To transfer a transgene from already developed transgenic line. Backcrossing is used
Stepwise transfer Simultaneous transfer Stepwise but parallel transfer Types of backcrossing when more than one gene is to be transferred from different sources
Conventional Backcross breeding P1 P1 P1 BC1F 1 P1 F 1 P2 BC2F 1 X X X P1 P1 BC3F 1 P1 X X BC4F 1 BC5F 1 BC6F 1 X X BC5- 98.4: 1.6 BC6- 99.2: 0.8
General equation for average of the recurrent parent: 1-(1/2)n+1 Where, n is the number of backcrosses to the recurrent parent. For f2, n=0 for BC1, n=1 for BC2, n=2 for BC3, n=3 etc.,
Problems of conventional backcrossing • Requires large number of plants for selection • Introgression of quantitative traits is nearly not possible. • Recovery of recipient genome is less efficient. • Poses difficulties in negative selection of undesirable genes (linkage drag problems) • Cannot select the plants until the traits are expressed. • Phenocopy effect hinders the selection. • Recessive traits take more time to transfer
Marker assisted breeding: application of molecular biotechnological tools, in combination with linkage maps and genomics, to improve plant or animal traits on the basis of genotypic assays.
Marker assisted backcrossing • Marker assisted backcrossing uses DNA markers, which can be scored as a dominant or codominant trait prior to flowering, to facilitate the backcrossing program, saving time if progeny testing would need to be conducted and saving resources if phenotyping is difficult. • Markers can be used to select for the gene being introgressed into the recurrent parent and to select against undesirable donor DNA other than the trait of interest. • Markers enable the pyramiding of resistance genes; they enable the incorporation of alleles at multiple loci each of which confers resistance to the same race of pathogen, which is difficult to do traditionally because one locus masks the presence of the others.
It is an approach that has been developed to avoid problems connected with conventional plant breeding by changing the selection criteria from selection of phenotypes towards selection of genes that control traits of interest, either directly or indirectly. MAB is the process of using the results of DNA tests to assist in the selection of individuals to become the parents in the next generation of a genetic improvement programme Principle of MAB:
The success of MAB depends upon: •The distance between the closest markers and the target gene, • Number of target genes to be transferred, • Genetic base of the trait, • Number of individuals that can be analyzed and the genetic background in which the target gene has to be transferred, •The type of molecular marker(s) used, and available technical facilities Factors responsible for the efficiency of MABC are- • Size of population for each backcross generation. • Markers distance from locus. • Number of markers is used in each selection process.
In Backcross Breeding, Markers Can Be Used To: I. Control the target gene (foreground selection) II. Control the genetic background (background selection). III.Control the linkage drag (recombinant selection)
✓Also known as positive selection- Proposed by Tanksley Foreground selection refers to the use of markers that are tightly linked to the gene of interest in order to select for the target allele or gene (associate a molecular marker with the target trait by some genetic mapping method). Foreground selection: 1 2 3 4 Target locus TARGET LOCUS SELECTION FOREGROUND SELECTION
The objective is to maintain the target locus in a heterozygous state (one donor allele and one RP allele) until the final backcross is completed. Then, the selected plants are self-pollinated and progeny plants identified that are homozygous for the donor allele. • markers may be used to screen for the target trait, which may be useful for traits that have laborious phenotypic screening procedures or recessive alleles. • Selection for target gene or QTL • Useful for traits that are difficult to evaluate • Also useful for recessive genes
Selecting backcross progeny with the target gene and tightly- linked flanking markers is termed as ‘recombinant selection •The purpose of recombinant selection is to reduce the size of the donor chromosome segment containing the target locus (i.e. size of the introgression). •Require large population sizes •By using markers that flank a target gene , linkage drag can be minimized. RECOMBINANT SELECTION 1 2 3 4 Recombinant Selection
1 2 3 4 BACKGROUND SELECTION ➢ Negative selection- Proposed by Takeuchi ➢ Background markers are markers that are unlinked to the target gene/QTL on all other chromosomes, in other words, markers that can be used to select against the donor genome. ➢ Background selection refers to the use of tightly linked flanking markers for recombinant selection and unlinked markers to select RP. ➢ This is extremely useful because the RP recovery can be greatly accelerated. Background Selection
• With conventional backcrossing, it takes a minimum of six BC generations to recover the RP and there may still be several donor chromosome fragments unlinked to the target gene. • The use of background selection during MABC to accelerate the development of an RP with an additional one or more genes has been referred to as ‘variety development or enhancement’ and ‘complete line conversion’ • Accelerates the recovery of the recurrent parent genome • Savings of 2, 3 or even 4 backcross generations
Schematic representation of development of resistant rice variety through marker-assisted backcrossing (MABC).
Schematic representation of selection of heterozygous carrying resistance gene based on genotyping analysis resembling RP genome at BC1F1.
Schematic representation of selection of heterozygous carrying resistance gene based on genotyping analysis resembling RP genome at BC2F1
Schematic representation of selection of homozygous plants for the donor allele
Schematic representation of transferring undesirable genes with target gene
Schematic representation of difference between conventional backcrossing and marker-assisted backcrossing
Comparison of conventional and Marker-Assisted backcrossing
Comparing the expected recovery of recurrent parent in conventional and Marker-Assisted backcrossing in subsequent generation. % of recurrent parent (RP) Backcross generation Number of Generation Marker-Assisted backcross Conventional backcross BC1 70 79.0 75.0 BC2 100 92.2 87.5 BC3 150 98.0 93.7 BC4 300 99.0 96.9 Hospital, 2003
Case studies
Super Annigeri 1 and improved JG 74: two Fusarium wilt-resistant introgression lines developed using marker-assisted backcrossing approach in chickpea (Cicer arietinum) Need to develop high yielding chickpea cultivars with FW resistance. Development of Super Annigeri 1 and improved JG 74 with enhanced yield and resistance to FW using MABC approach. Materials : Recipient parents – Annigeri 1 and JG74 ( susceptible to FW race 4) Donor parent – WR 315 (resistant to FW race 4) Mannur et al ., 2019
Annigeri 1 BC1F1 WR 315 BC2F1 X X BC2F2 BC2F3 X F1 Annigeri 1 Annigeri 1 BC2F4 in wilt sick plot X X X Hybridity confirmation 42 plants heterozygous for FG markers 38 SSRs for BGS, 80-87% RPGR 67 plants heterozygous for FG markers 35 SSRs for BGS, 90-95% RPGR 119 Plants showed resistance to FW resistant lines with higher yield Multi-locational phenotyping 2 superior lines Mannur et al ., 2019 Phenotyped for FW, resistant plants were obtained
Phenotypic evaluation for Fusarium Wilt disease Mannur et al ., 2019
JG 74 BC1F1 WR 315 BC2F1 X X BC3F1 BC3F2 X F1 Phenotyped for FW, 44 resistant plants were obtained BC3F4 in wilt sick plot X X Hybridity confirmation 3 plants heterozygous for FG markers 15 plants heterozygous for FG markers 42 SSRs for BGS, 52-97% RPGR JG 74 type plants were selected resistant lines with recurrent parent type 2 superior lines JG 74315-14 (MLT) JG 74 JG 74 X JG 74 BC3F3 X 4 plants heterozygous for FG markers JG 74315-2 & 14 evaluated Mannur et al ., 2019
Marker-Assisted Backcrossing to Introgress Resistance to Fusarium Wilt Race 1 and Ascochyta Blight in C 214, an Elite Cultivar of Chickpea Varshney et al ., 2014 Materials: 2 parallel crossing; C214 – recurrent parent ( susceptible to FW and AB disease) WR 315 – donor parent ( resistant to FW disease) ILC3279 – donor parent ( resistant to AB disease)
C 214 BC1F1 WR 315 BC2F1 X X BC3F1 BC3F2 X F1 BC3F4 X X Hybridity confirmation 41 plants heterozygous for FG markers 30 plants heterozygous for FG markers40 SSRs for BGS, 90-98%RPGR 98% RPGR homozygous plants with >98%rpgr C 214 C 214 X C 214 BC3F3 X Fusarium Wilt Varshney et al ., 2014 30 plants heterozygous for FGmarkers 32 SSR markers BGS, 89-95% RPGR
Screening of marker-assisted backcrossing (MABC) lines for resistance to Fusarium wilt
Disease reaction of parental and BC3F4 lines resistance to Fusarium oxysporum. Lines FW incidence (%) Disease reaction† Parental lines C 214 (recurrent parent) 54.50 susceptible WR 315 (donor parent) 6 resistant MABC lines‡ ICCX-100175-349-2-2 0 resistant ICCX-100175-389-3-2 5 resistant ICCX-100175-382-4-6 20 resistant
C 214 BC1F1 IL 3279 BC2F1 X X BC3F1 BC3F2 X F1 BC3F4 X X Hybridity confirmation 2 plants heterozygous for FG markers 38 plants heterozygous for FG markers 43 SSRs for BGS, 80-90% RPGR homozygous plants with >90%rpgr C 214 C 214 X C 214 BC3F3 X 46 plants heterozygous for FG markers 29 SSR markers BGS, 80-87% RPGR Ascochyta Blight Varshney et al ., 2014
Screening of marker-assisted backcrossing (MABC) lines for resistance to Ascochyta blight.
Disease reaction of parental and BC3F4 lines resistance to Ascochyta blight (AB). Lines AB score Disease reaction Parental lines C 214 (recurrent parent) 7 susceptible ILC 3279 (donor parent) 4 moderately resistant MABC lines ICCX-100176-421-1-11 3 resistant ICCX-100176-421-1-12 2 resistant ICCX-100176-470-2-5 2 resistant ICCX-100176-470-2-7 2 resistant ICCX-100176-470-2-16 3 resistant ICCX-100176-470-3-1 2 resistant ICCX-100176-470-3-3 3 resistant
Marker-Assisted Backcrossing to develop an Elite Cytoplasmic Male Sterility line in Rice To transfer CMS from IR68897 A line to Yosen B as a putative maintainer line, with the ultimate goal of application of the resultant final CMS line in hybrid rice seed production. Materials: Yosen B line – potential maintainer line for rice WA-CMS ( paternal recipient parent) CMS IR68897 A –maternal CMS donor parent Conducted Pollen fertility test from F1 generation to BC4F1 progenies. Foreground selection by using mitochondrial WA-CMS-specific marker for validating the transfer of CMS from donor to F1 hybrid and subsequent backcross progenies. Ahmadikhan et al ., 2015
IR68897-A BC1F1 F 1 Yosen-B 2 BC2F1 X X X 1 BC3F1 BC4F1 X X Yosen-B Yosen-B Yosen-B Yosen-B Tracing transfer of CMS higher RPG higher RPG 4 CMS plants with >98%RPG
Future prospects An efficient cost effective MABC technology must be developed that will allow breeders to assess the genotype across the full genome and to recombine genes of agronomic importance from diverse sources. The most significant cost prior MABC is the development of genetic linkage map for the species of interest.
MABC approach plays a vital role for basic research applications to develop new and advance varieties with much greater precision than conventional backcrossing. It has generated good deal of expectation, which in some cases let to over/optimize and in other to disappointment because many of the expectation have not been realized. Conclusion

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Marker assisted back cross

  • 1. Marker Assisted Backcross Breeding (MABC) in Crop Improvement
  • 2. ●Introduction ●Backcross breeding & its types ●Marker assisted breeding ●Marker assisted backcross breeding (MABC) ●Main strategies ●Advantages over conventional breeding ●Case studies ●Future outlook ●Conclusion Flow of seminar
  • 3. ● Backcross breeding is a well-known procedure for the introgression of a target gene f ● The objective is to reduce the donor genome content (DGC) of the progenies by repe Backcrossing 6
  • 4. Factors necessary for backcross method: (i) Recurrent parent Selection (ii) Screening for target trait (iii) Number of backcrosses ●To transfer a major gene ● In disease/pest resistance breeding ● To transfer alien cytoplasm or to transfer cytoplasmic male sterility ●To transfer a transgene from already developed transgenic line. Backcrossing is used
  • 5. Stepwise transfer Simultaneous transfer Stepwise but parallel transfer Types of backcrossing when more than one gene is to be transferred from different sources
  • 6. Conventional Backcross breeding P1 P1 P1 BC1F 1 P1 F 1 P2 BC2F 1 X X X P1 P1 BC3F 1 P1 X X BC4F 1 BC5F 1 BC6F 1 X X BC5- 98.4: 1.6 BC6- 99.2: 0.8
  • 7. General equation for average of the recurrent parent: 1-(1/2)n+1 Where, n is the number of backcrosses to the recurrent parent. For f2, n=0 for BC1, n=1 for BC2, n=2 for BC3, n=3 etc.,
  • 8. Problems of conventional backcrossing • Requires large number of plants for selection • Introgression of quantitative traits is nearly not possible. • Recovery of recipient genome is less efficient. • Poses difficulties in negative selection of undesirable genes (linkage drag problems) • Cannot select the plants until the traits are expressed. • Phenocopy effect hinders the selection. • Recessive traits take more time to transfer
  • 9. Marker assisted breeding: application of molecular biotechnological tools, in combination with linkage maps and genomics, to improve plant or animal traits on the basis of genotypic assays.
  • 10. Marker assisted backcrossing • Marker assisted backcrossing uses DNA markers, which can be scored as a dominant or codominant trait prior to flowering, to facilitate the backcrossing program, saving time if progeny testing would need to be conducted and saving resources if phenotyping is difficult. • Markers can be used to select for the gene being introgressed into the recurrent parent and to select against undesirable donor DNA other than the trait of interest. • Markers enable the pyramiding of resistance genes; they enable the incorporation of alleles at multiple loci each of which confers resistance to the same race of pathogen, which is difficult to do traditionally because one locus masks the presence of the others.
  • 11. It is an approach that has been developed to avoid problems connected with conventional plant breeding by changing the selection criteria from selection of phenotypes towards selection of genes that control traits of interest, either directly or indirectly. MAB is the process of using the results of DNA tests to assist in the selection of individuals to become the parents in the next generation of a genetic improvement programme Principle of MAB:
  • 12. The success of MAB depends upon: •The distance between the closest markers and the target gene, • Number of target genes to be transferred, • Genetic base of the trait, • Number of individuals that can be analyzed and the genetic background in which the target gene has to be transferred, •The type of molecular marker(s) used, and available technical facilities Factors responsible for the efficiency of MABC are- • Size of population for each backcross generation. • Markers distance from locus. • Number of markers is used in each selection process.
  • 13. In Backcross Breeding, Markers Can Be Used To: I. Control the target gene (foreground selection) II. Control the genetic background (background selection). III.Control the linkage drag (recombinant selection)
  • 14. ✓Also known as positive selection- Proposed by Tanksley Foreground selection refers to the use of markers that are tightly linked to the gene of interest in order to select for the target allele or gene (associate a molecular marker with the target trait by some genetic mapping method). Foreground selection: 1 2 3 4 Target locus TARGET LOCUS SELECTION FOREGROUND SELECTION
  • 15. The objective is to maintain the target locus in a heterozygous state (one donor allele and one RP allele) until the final backcross is completed. Then, the selected plants are self-pollinated and progeny plants identified that are homozygous for the donor allele. • markers may be used to screen for the target trait, which may be useful for traits that have laborious phenotypic screening procedures or recessive alleles. • Selection for target gene or QTL • Useful for traits that are difficult to evaluate • Also useful for recessive genes
  • 16. Selecting backcross progeny with the target gene and tightly- linked flanking markers is termed as ‘recombinant selection •The purpose of recombinant selection is to reduce the size of the donor chromosome segment containing the target locus (i.e. size of the introgression). •Require large population sizes •By using markers that flank a target gene , linkage drag can be minimized. RECOMBINANT SELECTION 1 2 3 4 Recombinant Selection
  • 17. 1 2 3 4 BACKGROUND SELECTION ➢ Negative selection- Proposed by Takeuchi ➢ Background markers are markers that are unlinked to the target gene/QTL on all other chromosomes, in other words, markers that can be used to select against the donor genome. ➢ Background selection refers to the use of tightly linked flanking markers for recombinant selection and unlinked markers to select RP. ➢ This is extremely useful because the RP recovery can be greatly accelerated. Background Selection
  • 18. • With conventional backcrossing, it takes a minimum of six BC generations to recover the RP and there may still be several donor chromosome fragments unlinked to the target gene. • The use of background selection during MABC to accelerate the development of an RP with an additional one or more genes has been referred to as ‘variety development or enhancement’ and ‘complete line conversion’ • Accelerates the recovery of the recurrent parent genome • Savings of 2, 3 or even 4 backcross generations
  • 19. Schematic representation of development of resistant rice variety through marker-assisted backcrossing (MABC).
  • 20. Schematic representation of selection of heterozygous carrying resistance gene based on genotyping analysis resembling RP genome at BC1F1.
  • 21. Schematic representation of selection of heterozygous carrying resistance gene based on genotyping analysis resembling RP genome at BC2F1
  • 22. Schematic representation of selection of homozygous plants for the donor allele
  • 23. Schematic representation of transferring undesirable genes with target gene
  • 24. Schematic representation of difference between conventional backcrossing and marker-assisted backcrossing
  • 25. Comparison of conventional and Marker-Assisted backcrossing
  • 26. Comparing the expected recovery of recurrent parent in conventional and Marker-Assisted backcrossing in subsequent generation. % of recurrent parent (RP) Backcross generation Number of Generation Marker-Assisted backcross Conventional backcross BC1 70 79.0 75.0 BC2 100 92.2 87.5 BC3 150 98.0 93.7 BC4 300 99.0 96.9 Hospital, 2003
  • 28. Super Annigeri 1 and improved JG 74: two Fusarium wilt-resistant introgression lines developed using marker-assisted backcrossing approach in chickpea (Cicer arietinum) Need to develop high yielding chickpea cultivars with FW resistance. Development of Super Annigeri 1 and improved JG 74 with enhanced yield and resistance to FW using MABC approach. Materials : Recipient parents – Annigeri 1 and JG74 ( susceptible to FW race 4) Donor parent – WR 315 (resistant to FW race 4) Mannur et al ., 2019
  • 29. Annigeri 1 BC1F1 WR 315 BC2F1 X X BC2F2 BC2F3 X F1 Annigeri 1 Annigeri 1 BC2F4 in wilt sick plot X X X Hybridity confirmation 42 plants heterozygous for FG markers 38 SSRs for BGS, 80-87% RPGR 67 plants heterozygous for FG markers 35 SSRs for BGS, 90-95% RPGR 119 Plants showed resistance to FW resistant lines with higher yield Multi-locational phenotyping 2 superior lines Mannur et al ., 2019 Phenotyped for FW, resistant plants were obtained
  • 30. Phenotypic evaluation for Fusarium Wilt disease Mannur et al ., 2019
  • 31. JG 74 BC1F1 WR 315 BC2F1 X X BC3F1 BC3F2 X F1 Phenotyped for FW, 44 resistant plants were obtained BC3F4 in wilt sick plot X X Hybridity confirmation 3 plants heterozygous for FG markers 15 plants heterozygous for FG markers 42 SSRs for BGS, 52-97% RPGR JG 74 type plants were selected resistant lines with recurrent parent type 2 superior lines JG 74315-14 (MLT) JG 74 JG 74 X JG 74 BC3F3 X 4 plants heterozygous for FG markers JG 74315-2 & 14 evaluated Mannur et al ., 2019
  • 32. Marker-Assisted Backcrossing to Introgress Resistance to Fusarium Wilt Race 1 and Ascochyta Blight in C 214, an Elite Cultivar of Chickpea Varshney et al ., 2014 Materials: 2 parallel crossing; C214 – recurrent parent ( susceptible to FW and AB disease) WR 315 – donor parent ( resistant to FW disease) ILC3279 – donor parent ( resistant to AB disease)
  • 33. C 214 BC1F1 WR 315 BC2F1 X X BC3F1 BC3F2 X F1 BC3F4 X X Hybridity confirmation 41 plants heterozygous for FG markers 30 plants heterozygous for FG markers40 SSRs for BGS, 90-98%RPGR 98% RPGR homozygous plants with >98%rpgr C 214 C 214 X C 214 BC3F3 X Fusarium Wilt Varshney et al ., 2014 30 plants heterozygous for FGmarkers 32 SSR markers BGS, 89-95% RPGR
  • 34. Screening of marker-assisted backcrossing (MABC) lines for resistance to Fusarium wilt
  • 35. Disease reaction of parental and BC3F4 lines resistance to Fusarium oxysporum. Lines FW incidence (%) Disease reaction† Parental lines C 214 (recurrent parent) 54.50 susceptible WR 315 (donor parent) 6 resistant MABC lines‡ ICCX-100175-349-2-2 0 resistant ICCX-100175-389-3-2 5 resistant ICCX-100175-382-4-6 20 resistant
  • 36. C 214 BC1F1 IL 3279 BC2F1 X X BC3F1 BC3F2 X F1 BC3F4 X X Hybridity confirmation 2 plants heterozygous for FG markers 38 plants heterozygous for FG markers 43 SSRs for BGS, 80-90% RPGR homozygous plants with >90%rpgr C 214 C 214 X C 214 BC3F3 X 46 plants heterozygous for FG markers 29 SSR markers BGS, 80-87% RPGR Ascochyta Blight Varshney et al ., 2014
  • 37. Screening of marker-assisted backcrossing (MABC) lines for resistance to Ascochyta blight.
  • 38. Disease reaction of parental and BC3F4 lines resistance to Ascochyta blight (AB). Lines AB score Disease reaction Parental lines C 214 (recurrent parent) 7 susceptible ILC 3279 (donor parent) 4 moderately resistant MABC lines ICCX-100176-421-1-11 3 resistant ICCX-100176-421-1-12 2 resistant ICCX-100176-470-2-5 2 resistant ICCX-100176-470-2-7 2 resistant ICCX-100176-470-2-16 3 resistant ICCX-100176-470-3-1 2 resistant ICCX-100176-470-3-3 3 resistant
  • 39. Marker-Assisted Backcrossing to develop an Elite Cytoplasmic Male Sterility line in Rice To transfer CMS from IR68897 A line to Yosen B as a putative maintainer line, with the ultimate goal of application of the resultant final CMS line in hybrid rice seed production. Materials: Yosen B line – potential maintainer line for rice WA-CMS ( paternal recipient parent) CMS IR68897 A –maternal CMS donor parent Conducted Pollen fertility test from F1 generation to BC4F1 progenies. Foreground selection by using mitochondrial WA-CMS-specific marker for validating the transfer of CMS from donor to F1 hybrid and subsequent backcross progenies. Ahmadikhan et al ., 2015
  • 40. IR68897-A BC1F1 F 1 Yosen-B 2 BC2F1 X X X 1 BC3F1 BC4F1 X X Yosen-B Yosen-B Yosen-B Yosen-B Tracing transfer of CMS higher RPG higher RPG 4 CMS plants with >98%RPG
  • 41. Future prospects An efficient cost effective MABC technology must be developed that will allow breeders to assess the genotype across the full genome and to recombine genes of agronomic importance from diverse sources. The most significant cost prior MABC is the development of genetic linkage map for the species of interest.
  • 42. MABC approach plays a vital role for basic research applications to develop new and advance varieties with much greater precision than conventional backcrossing. It has generated good deal of expectation, which in some cases let to over/optimize and in other to disappointment because many of the expectation have not been realized. Conclusion