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Molecular markers for measuring genetic 
diversity 
Introduction: 
The molecular basis of the essential biological phenomena in plants is crucial for the effective 
conservation, management, and efficient utilization of plant genetic resources (PGR). 
Determining genetic diversity can be based on morphological, biochemical, and molecular types 
of information. However, molecular markers have advantages over other kinds, where they show 
genetic differences on a more detailed level without interferences from environmental factors, 
and where they involve techniques that provide fast results detailing genetic diversity 
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Comparison of different methods 
 Morphological characterization does not require expensive technology but large tracts of 
land are often required for these experiments, making it possibly more expensive than 
molecular assessment. These traits are often susceptible to phenotypic plasticity; conversely, 
this allows assessment of diversity in the presence of environmental variation. 
 Biochemical analysis is based on the separation of proteins into specific banding patterns. It 
is a fast method which requires only small amounts of biological material. However, only a 
limited number of enzymes are available and thus, the resolution of diversity is limited. 
 Molecular analyses comprise a large variety of DNA molecular markers, which can be 
employed for analysis of variation. Different markers have different genetic qualities (they 
can be dominant or co-dominant, can amplify anonymous or characterized loci, can contain 
expressed or non-expressed sequences, etc.). 
Genetic marker 
The concept of genetic markers is not a new one; in the nineteenth century, Gregor Mendel 
employed phenotype-based genetic markers in his experiments. Later, phenotype-based genetic 
markers for Drosophila melanogaster led to the founding of the theory of genetic linkage. 
A genetic marker is an easily identifiable piece of genetic material, usually DNA that can be 
used in the laboratory to tell apart cells, individuals, populations, or species. 
The use of genetic markers begins with extracting proteins or chemicals (for biochemical 
markers) or DNA (for molecular markers) from tissues of the plant (for example, seeds, foliage, 
pollen, sometimes woody tissues). 
Molecular markers 
In genetics, a molecular marker (identified as genetic marker) is a fragment of DNA that is
2 
associated with a certain location within the genome. 
Molecular markers which detect variation at the DNA level such as nucleotide changes: deletion, 
duplication, inversion and/or insertion. Markers can exhibit two modes of inheritance, i.e. 
dominant/recessive or co-dominant. If the genetic pattern of homozygotes can be distinguished 
from that of heterozygotes, then a marker is said to be co-dominant. Generally co-dominant 
markers are more informative than the dominant markers. 
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Characteristics of molecular marker 
 Be polymorphic and evenly distributed throughout the genome. 
 Provide adequate resolution of genetic differences. 
 Generate multiple, independent and reliable markers. 
 Be simple, quick and inexpensive. 
 Need small amounts of tissue and DNA samples. 
 Link to distinct phenotypes. 
 Require no prior Diversity information about the genome of an organism. 
Advantages of molecular marker 
 Being applicable to any part of the genome (introns, exons and regulation regions). 
 Not possessing pleiotrophic or epistatic effects. 
 Being able to distinguish polymorphisms which not produce phenotypic variation and 
finally. 
 Being some of them co-dominant. 
Types of molecular markers 
Basic marker techniques can be classified into two categories: 
(1) non-PCR-based techniques or hybridization based techniques. 
(2) PCR-based techniques. 
1. Randomly Amplified Polymorphic DNA (RAPD) 
RAPD was the first PCR based molecular marker technique developed and it is by far the 
simplest Short PCR primers (approximately 10 bases) are randomly and arbitrarily selected to 
amplify random DNA segments throughout the genome. The resulting amplification product is 
generated at the region flanking a part of the 10 bp priming sites in the appropriate orientation. 
RAPD products are usually visualized on agarose gels stained with ethedium bromide.
3 
RAPD markers are easily developed and because they are based on PCR amplification followed 
by agarose gel electrophoresis, they are quickly and readily detected. RAPD technique was used 
extensively in studying genetic diversity between plant species. For example, it was used to 
study genetic structure and diversity among and between six populations of Capparis deciduas in 
Saudi Arabia. 
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2. Amplified Fragment Length Polymorphisms (AFLP) 
Amplified Fragment Length Polymorphisms (AFLP) based genomic DNA fingerprinting is a 
technique used to detect DNA polymorphism. AFLP is a polymerase chain reaction (PCR) based 
technique, has been reliably used for determining genetic diversity and phylogenetic relationship 
between closely related genotypes. AFLP markers are generally dominant and do not require 
prior knowledge of the genomic composition. AFLPs are produced in great numbers and are 
reproducible 
The AFLP is applicable to all species giving very reproducible results. It was also used in 
microbial population: in studying genetic diversity of human pathogenic bacteria. In that regards 
it has the advantage of the extensive coverage of the genome under study. In addition the 
complexity of the bands can be reduced by adding selective bases to the primers during PCR 
amplification. It was also used in studying genetic diversity of human pathogenic bacteria the 
completion of the genome sequencing of E. coli, it was possible to predict the band pattern of the 
AFLP analysis of E. coli. This indicates the power of this technique. In higher plants AFLP was 
used in variety of applications which includes examining genetic relationship between species 
investigating genetic structure of gene pool and assessment of genetic differentiation among 
populations 
3. Single nucleotide polymorphism SNP’s 
Single nucleotide polymorphism SNP’s, represent sites in the genome where DNA sequence 
differs by a single base when two or more individuals are compared. They may be individually 
responsible for specific traits or phenotypes, or may represent neutral variation that is useful for 
evaluating diversity in the context of evolution. SNPs are the most widespread type of sequence 
variation in genomes discovered so far. About 90% of sequence variants in humans are 
differences in single bases of DNA 
Several disciplines such as population ecology and conservation and evolutionary genetics are 
benefitting from SNPs as genetic markers. There is widespread interest in finding SNP’s because 
they are numerous, more stable, potentially easier to score than the microsatellite repeats 
currently been used in gene mapping in human. Within coding regions there are on average four 
SNPs per gene with a frequency above 1%. About half of these cause amino acid substitutions: 
termed non-synonymous SNPs
4 
Because of the importance of the SNP’s in the discovery of DNA sequence variants, the National 
Human Genome Research Institute (NHGRI) of NIH along with the Center for Disease Control 
and Prevention and several individual investigators have assembled a DNA Polymorphism 
Discovery Resource of samples from 450 U.S. residents This DNA variant discovery will help in 
finding SNP’s that are deleterious to gene function or likely to be disease associated. 
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4. Microsatellite-Based Marker Technique 
Microsatellites or Simple Sequence Repeats (SSR) are sets repeated sequences found within 
eukaryotic These consist of sequences of repetitions, comprising basic short motifs generally 
between 2 and 6 base-pairs long. Polymorphisms associated with a specific locus are due to the 
variation in length of the microsatellite, which in turn depends on the number of repetitions of 
the basic motif. Variations in the number of tandemly repeated units are mainly due to strand 
slippage during DNA replication where the repeats allow matching via excision or addition of 
repeats. As slippage in replication is more likely than point mutations, microsatellite loci tend to 
be hypervariable. 
Microsatellite assays show extensive inter-individual length polymorphisms during PCR analysis 
of unique loci using discriminatory primers sets. Microsatellites are highly popular genetic 
markers as they possess: co-dominant inheritance, high abundance, enormous extent of allelic 
diversity, ease of assessing SSR size variation through PCR with pairs of flanking primers and 
high reproducibility. However, the development of microsatellites requires extensive knowledge 
of DNA sequences, and sometimes they underestimate genetic structure measurements, hence 
they have been developed primarily for agricultural species, rather than wild species. Initial 
approaches were principally based on hybridization techniques, whilst more recent techniques 
are based on PCR. 
Major molecular markers based on assessment of variability generated by microsatellites 
sequences are: STMSs (Sequence Tagged Microsatellite Site), SSLPs (Simple Sequence Length 
Polymorphism), SNPs (Single Nucleotide Polymorphisms), SCARs (Sequence Characterized 
Amplified Region) and CAPS (Cleaved Amplified Polymorphic Sequences) 
5. Restriction-Hybridization Techniques (Non-PCR-Based) 
Molecular markers based on restriction-hybridization techniques were employed relatively 
early in the field of plant studies and combined the use of restriction endonucleases and the 
hybridization method. Restriction endonucleases are bacterial enzymes able to cut DNA, 
identifying specific palindrome sequences and producing polynucleotidic fragments with 
variable dimensions. Any changes within sequences (i.e., point mutations), mutations between 
two sites (i.e., deletions and translocations), or mutations within the enzyme site, can generate 
variations in the length of restriction fragment obtained after enzymatic digestion.
5 
RFLP and Variable Numbers of Tandem Repeats (VNTRs) markers are examples of molecular 
markers based on restriction-hybridization techniques. In RFLP, DNA polymorphism is detected 
by hybridizing a chemically-labelled DNA probe to a Southern blot of DNA digested by 
restriction endonucleases, resulting in differential DNA fragment profile. The RFLP markers are 
relatively highly polymorphic, codominantly inherited, and highly replicable and allow the 
simultaneously screening of numerous samples. DNA blots can be analyzed repeatedly by 
stripping and reprobing (usually eight to ten times) with different RFLP probes. Nevertheless, 
this technique is not very widely used as it is time-consuming, involves expensive and 
radioactive/toxic reagents and requires large quantities of high quality genomic DNA. Moreover, 
the prerequisite of prior sequence information for probe construction contributes to the 
complexity of the methodology. These limitations led to the development of a new set of less 
technically complex methods known as PCR-based techniques. 
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Molecular markers for measuring genetic diversity

  • 1. 1 Molecular markers for measuring genetic diversity Introduction: The molecular basis of the essential biological phenomena in plants is crucial for the effective conservation, management, and efficient utilization of plant genetic resources (PGR). Determining genetic diversity can be based on morphological, biochemical, and molecular types of information. However, molecular markers have advantages over other kinds, where they show genetic differences on a more detailed level without interferences from environmental factors, and where they involve techniques that provide fast results detailing genetic diversity Sp13-bty-001 Comparison of different methods  Morphological characterization does not require expensive technology but large tracts of land are often required for these experiments, making it possibly more expensive than molecular assessment. These traits are often susceptible to phenotypic plasticity; conversely, this allows assessment of diversity in the presence of environmental variation.  Biochemical analysis is based on the separation of proteins into specific banding patterns. It is a fast method which requires only small amounts of biological material. However, only a limited number of enzymes are available and thus, the resolution of diversity is limited.  Molecular analyses comprise a large variety of DNA molecular markers, which can be employed for analysis of variation. Different markers have different genetic qualities (they can be dominant or co-dominant, can amplify anonymous or characterized loci, can contain expressed or non-expressed sequences, etc.). Genetic marker The concept of genetic markers is not a new one; in the nineteenth century, Gregor Mendel employed phenotype-based genetic markers in his experiments. Later, phenotype-based genetic markers for Drosophila melanogaster led to the founding of the theory of genetic linkage. A genetic marker is an easily identifiable piece of genetic material, usually DNA that can be used in the laboratory to tell apart cells, individuals, populations, or species. The use of genetic markers begins with extracting proteins or chemicals (for biochemical markers) or DNA (for molecular markers) from tissues of the plant (for example, seeds, foliage, pollen, sometimes woody tissues). Molecular markers In genetics, a molecular marker (identified as genetic marker) is a fragment of DNA that is
  • 2. 2 associated with a certain location within the genome. Molecular markers which detect variation at the DNA level such as nucleotide changes: deletion, duplication, inversion and/or insertion. Markers can exhibit two modes of inheritance, i.e. dominant/recessive or co-dominant. If the genetic pattern of homozygotes can be distinguished from that of heterozygotes, then a marker is said to be co-dominant. Generally co-dominant markers are more informative than the dominant markers. Sp13-bty-001 Characteristics of molecular marker  Be polymorphic and evenly distributed throughout the genome.  Provide adequate resolution of genetic differences.  Generate multiple, independent and reliable markers.  Be simple, quick and inexpensive.  Need small amounts of tissue and DNA samples.  Link to distinct phenotypes.  Require no prior Diversity information about the genome of an organism. Advantages of molecular marker  Being applicable to any part of the genome (introns, exons and regulation regions).  Not possessing pleiotrophic or epistatic effects.  Being able to distinguish polymorphisms which not produce phenotypic variation and finally.  Being some of them co-dominant. Types of molecular markers Basic marker techniques can be classified into two categories: (1) non-PCR-based techniques or hybridization based techniques. (2) PCR-based techniques. 1. Randomly Amplified Polymorphic DNA (RAPD) RAPD was the first PCR based molecular marker technique developed and it is by far the simplest Short PCR primers (approximately 10 bases) are randomly and arbitrarily selected to amplify random DNA segments throughout the genome. The resulting amplification product is generated at the region flanking a part of the 10 bp priming sites in the appropriate orientation. RAPD products are usually visualized on agarose gels stained with ethedium bromide.
  • 3. 3 RAPD markers are easily developed and because they are based on PCR amplification followed by agarose gel electrophoresis, they are quickly and readily detected. RAPD technique was used extensively in studying genetic diversity between plant species. For example, it was used to study genetic structure and diversity among and between six populations of Capparis deciduas in Saudi Arabia. Sp13-bty-001 2. Amplified Fragment Length Polymorphisms (AFLP) Amplified Fragment Length Polymorphisms (AFLP) based genomic DNA fingerprinting is a technique used to detect DNA polymorphism. AFLP is a polymerase chain reaction (PCR) based technique, has been reliably used for determining genetic diversity and phylogenetic relationship between closely related genotypes. AFLP markers are generally dominant and do not require prior knowledge of the genomic composition. AFLPs are produced in great numbers and are reproducible The AFLP is applicable to all species giving very reproducible results. It was also used in microbial population: in studying genetic diversity of human pathogenic bacteria. In that regards it has the advantage of the extensive coverage of the genome under study. In addition the complexity of the bands can be reduced by adding selective bases to the primers during PCR amplification. It was also used in studying genetic diversity of human pathogenic bacteria the completion of the genome sequencing of E. coli, it was possible to predict the band pattern of the AFLP analysis of E. coli. This indicates the power of this technique. In higher plants AFLP was used in variety of applications which includes examining genetic relationship between species investigating genetic structure of gene pool and assessment of genetic differentiation among populations 3. Single nucleotide polymorphism SNP’s Single nucleotide polymorphism SNP’s, represent sites in the genome where DNA sequence differs by a single base when two or more individuals are compared. They may be individually responsible for specific traits or phenotypes, or may represent neutral variation that is useful for evaluating diversity in the context of evolution. SNPs are the most widespread type of sequence variation in genomes discovered so far. About 90% of sequence variants in humans are differences in single bases of DNA Several disciplines such as population ecology and conservation and evolutionary genetics are benefitting from SNPs as genetic markers. There is widespread interest in finding SNP’s because they are numerous, more stable, potentially easier to score than the microsatellite repeats currently been used in gene mapping in human. Within coding regions there are on average four SNPs per gene with a frequency above 1%. About half of these cause amino acid substitutions: termed non-synonymous SNPs
  • 4. 4 Because of the importance of the SNP’s in the discovery of DNA sequence variants, the National Human Genome Research Institute (NHGRI) of NIH along with the Center for Disease Control and Prevention and several individual investigators have assembled a DNA Polymorphism Discovery Resource of samples from 450 U.S. residents This DNA variant discovery will help in finding SNP’s that are deleterious to gene function or likely to be disease associated. Sp13-bty-001 4. Microsatellite-Based Marker Technique Microsatellites or Simple Sequence Repeats (SSR) are sets repeated sequences found within eukaryotic These consist of sequences of repetitions, comprising basic short motifs generally between 2 and 6 base-pairs long. Polymorphisms associated with a specific locus are due to the variation in length of the microsatellite, which in turn depends on the number of repetitions of the basic motif. Variations in the number of tandemly repeated units are mainly due to strand slippage during DNA replication where the repeats allow matching via excision or addition of repeats. As slippage in replication is more likely than point mutations, microsatellite loci tend to be hypervariable. Microsatellite assays show extensive inter-individual length polymorphisms during PCR analysis of unique loci using discriminatory primers sets. Microsatellites are highly popular genetic markers as they possess: co-dominant inheritance, high abundance, enormous extent of allelic diversity, ease of assessing SSR size variation through PCR with pairs of flanking primers and high reproducibility. However, the development of microsatellites requires extensive knowledge of DNA sequences, and sometimes they underestimate genetic structure measurements, hence they have been developed primarily for agricultural species, rather than wild species. Initial approaches were principally based on hybridization techniques, whilst more recent techniques are based on PCR. Major molecular markers based on assessment of variability generated by microsatellites sequences are: STMSs (Sequence Tagged Microsatellite Site), SSLPs (Simple Sequence Length Polymorphism), SNPs (Single Nucleotide Polymorphisms), SCARs (Sequence Characterized Amplified Region) and CAPS (Cleaved Amplified Polymorphic Sequences) 5. Restriction-Hybridization Techniques (Non-PCR-Based) Molecular markers based on restriction-hybridization techniques were employed relatively early in the field of plant studies and combined the use of restriction endonucleases and the hybridization method. Restriction endonucleases are bacterial enzymes able to cut DNA, identifying specific palindrome sequences and producing polynucleotidic fragments with variable dimensions. Any changes within sequences (i.e., point mutations), mutations between two sites (i.e., deletions and translocations), or mutations within the enzyme site, can generate variations in the length of restriction fragment obtained after enzymatic digestion.
  • 5. 5 RFLP and Variable Numbers of Tandem Repeats (VNTRs) markers are examples of molecular markers based on restriction-hybridization techniques. In RFLP, DNA polymorphism is detected by hybridizing a chemically-labelled DNA probe to a Southern blot of DNA digested by restriction endonucleases, resulting in differential DNA fragment profile. The RFLP markers are relatively highly polymorphic, codominantly inherited, and highly replicable and allow the simultaneously screening of numerous samples. DNA blots can be analyzed repeatedly by stripping and reprobing (usually eight to ten times) with different RFLP probes. Nevertheless, this technique is not very widely used as it is time-consuming, involves expensive and radioactive/toxic reagents and requires large quantities of high quality genomic DNA. Moreover, the prerequisite of prior sequence information for probe construction contributes to the complexity of the methodology. These limitations led to the development of a new set of less technically complex methods known as PCR-based techniques. Sp13-bty-001