AI Article Synopsis

  • - High-throughput sequencing is being tested as a more effective method for genotyping microsatellites compared to traditional capillary electrophoresis, addressing issues like amplification artifacts and imprecise sizing.
  • - In a study involving 180 muskrat specimens, sequencing revealed 294 alleles, unlike capillary electrophoresis, which would have only detected 164 due to length homoplasy, enabling better understanding of population genetics.
  • - The advantages of this sequencing method include precise fragment sizing and the ability to analyze many samples together, though it is most cost-effective when processing a large number of samples at once, highlighting the need for future improvements in cost-efficiency and data analysis tools.

Article Abstract

High-throughput sequencing has been proposed as a method to genotype microsatellites and overcome the four main technical drawbacks of capillary electrophoresis: amplification artifacts, imprecise sizing, length homoplasy, and limited multiplex capability. The objective of this project was to test a high-throughput amplicon sequencing approach to fragment analysis of short tandem repeats and characterize its advantages and disadvantages against traditional capillary electrophoresis. We amplified and sequenced 12 muskrat microsatellite loci from 180 muskrat specimens and analyzed the sequencing data for precision of allele calling, propensity for amplification or sequencing artifacts, and for evidence of length homoplasy. Of the 294 total alleles, we detected by sequencing, only 164 alleles would have been detected by capillary electrophoresis as the remaining 130 alleles (44%) would have been hidden by length homoplasy. The ability to detect a greater number of unique alleles resulted in the ability to resolve greater population genetic structure. The primary advantages of fragment analysis by sequencing are the ability to precisely size fragments, resolve length homoplasy, multiplex many individuals and many loci into a single high-throughput run, and compare data across projects and across laboratories (present and future) with minimal technical calibration. A significant disadvantage of fragment analysis by sequencing is that the method is only practical and cost-effective when performed on batches of several hundred samples with multiple loci. Future work is needed to optimize throughput while minimizing costs and to update existing microsatellite allele calling and analysis programs to accommodate sequence-aware microsatellite data.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC4930997PMC
http://dx.doi.org/10.1002/ece3.2221DOI Listing

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