TY - JOUR
T1 - Optimized PCR conditions minimizing the formation of chimeric DNA molecules from MPRA plasmid libraries
AU - Omelina, Evgeniya S.
AU - Ivankin, Anton V.
AU - Letiagina, Anna E.
AU - Pindyurin, Alexey V.
N1 - Publisher Copyright:
© 2019 The Author(s).
PY - 2019/7/11
Y1 - 2019/7/11
N2 - Background: Massively parallel reporter assays (MPRAs) enable high-throughput functional evaluation of various DNA regulatory elements and their mutant variants. The assays are based on construction of highly diverse plasmid libraries containing two variable fragments, a region of interest (a sequence under study; ROI) and a barcode (BC) used to uniquely tag each ROI, which are separated by a constant spacer sequence. The sequences of BC-ROI combinations present in the libraries may be either known a priori or not. In the latter case, it is necessary to identify these combinations before performing functional experiments. Typically, this is done by PCR amplification of the BC-ROI regions with flanking primers, followed by next-generation sequencing (NGS) of the products. However, chimeric DNA molecules formed on templates with identical spacer fragment during the amplification process may substantially hamper the identification of genuine BC-ROI combinations, and as a result lower the performance of the assays. Results: To identify settings that minimize formation of chimeric products we tested a number of PCR amplification parameters, such as conventional and emulsion types of PCR, one- or two-round amplification strategies, amount of DNA template, number of PCR cycles, and the duration of the extension step. Using specific MPRA libraries as templates, we found that the two-round amplification of the BC-ROI regions with a very low initial template amount, an elongated extension step, and a specific number of PCR cycles result in as low as 0.30 and 0.32% of chimeric products for emulsion and conventional PCR approaches, respectively. Conclusions: We have identified PCR parameters that ensure synthesis of specific (non-chimeric) products from highly diverse MPRA plasmid libraries. In addition, we found that there is a negligible difference in performance of emulsion and conventional PCR approaches performed with the identified settings.
AB - Background: Massively parallel reporter assays (MPRAs) enable high-throughput functional evaluation of various DNA regulatory elements and their mutant variants. The assays are based on construction of highly diverse plasmid libraries containing two variable fragments, a region of interest (a sequence under study; ROI) and a barcode (BC) used to uniquely tag each ROI, which are separated by a constant spacer sequence. The sequences of BC-ROI combinations present in the libraries may be either known a priori or not. In the latter case, it is necessary to identify these combinations before performing functional experiments. Typically, this is done by PCR amplification of the BC-ROI regions with flanking primers, followed by next-generation sequencing (NGS) of the products. However, chimeric DNA molecules formed on templates with identical spacer fragment during the amplification process may substantially hamper the identification of genuine BC-ROI combinations, and as a result lower the performance of the assays. Results: To identify settings that minimize formation of chimeric products we tested a number of PCR amplification parameters, such as conventional and emulsion types of PCR, one- or two-round amplification strategies, amount of DNA template, number of PCR cycles, and the duration of the extension step. Using specific MPRA libraries as templates, we found that the two-round amplification of the BC-ROI regions with a very low initial template amount, an elongated extension step, and a specific number of PCR cycles result in as low as 0.30 and 0.32% of chimeric products for emulsion and conventional PCR approaches, respectively. Conclusions: We have identified PCR parameters that ensure synthesis of specific (non-chimeric) products from highly diverse MPRA plasmid libraries. In addition, we found that there is a negligible difference in performance of emulsion and conventional PCR approaches performed with the identified settings.
KW - Barcode
KW - Chimeric DNA molecules
KW - Conventional PCR
KW - Emulsion PCR (ePCR)
KW - Massively parallel reporter assay (MPRA)
KW - Next-generation sequencing
KW - SEQUENCES
KW - CIS-REGULATORY FUNCTION
KW - COAMPLIFICATION
KW - IDENTIFICATION
KW - RIBOSOMAL-RNA GENES
KW - AMPLIFICATION
KW - DISSECTION
KW - MEDIATED RECOMBINATION
KW - CONSEQUENCE
KW - FREQUENCY
UR - http://www.scopus.com/inward/record.url?scp=85069044029&partnerID=8YFLogxK
U2 - 10.1186/s12864-019-5847-2
DO - 10.1186/s12864-019-5847-2
M3 - Article
C2 - 31291895
AN - SCOPUS:85069044029
VL - 20
SP - 536
JO - BMC Genomics
JF - BMC Genomics
SN - 1471-2164
IS - Suppl 7
M1 - 536
ER -