Quantification of ssDNA Scaffold Production by Ion-Pair Reverse Phase Chromatography

被引：0

作者：

Silva-Santos, A. Rita ^{[1
,2
]}

Rosa, Sara Sousa ^{[1
,2
]}

Marques, Marco P. C. ^{[3
]}

Azevedo, Ana M. ^{[1
,2
]}

Prazeres, Duarte Miguel F. ^{[1
,2
]}

机构：

[1] Univ Lisbon, iBB Inst Bioengn & Biosci, Dept Bioengn, Inst Super Tecn, P-1049001 Lisbon, Portugal

[2] Univ Lisbon, Inst Hlth & Bioecon, Associate Lab i4HB, Inst Super Tecn, P-1049001 Lisbon, Portugal

[3] UCL, Dept Biochem Engn, London WC1H 0AH, England

来源：

ACS OMEGA | 2024年 / 9卷 / 21期

基金：

英国工程与自然科学研究理事会; 英国生物技术与生命科学研究理事会;

关键词：

SINGLE-STRANDED-DNA; LIQUID-CHROMATOGRAPHY; MASS-SPECTROMETRY; FRAGMENTS;

D O I：

10.1021/acsomega.3c10533

中图分类号：

O6 [化学];

学科分类号：

0703 ;

摘要：

DNA origami is an emerging technology that can be used as a nanoscale platform in numerous applications ranging from drug delivery systems to biosensors. The DNA nanostructures are assembled from large single-stranded DNA (ssDNA) scaffolds, ranging from hundreds to thousands of nucleotides and from short staple strands. Scaffolds are usually obtained by asymmetric PCR (aPCR) or Escherichia coli infection/transformation with phages or phagemids. Scaffold quantification is typically based on agarose gel electrophoresis densitometry for molecules obtained by aPCR, or by UV absorbance, in the case of scaffolds obtained by infection or transformation. Although these methods are well-established and easy-to-apply, the results obtained are often inaccurate due to the lack of selectivity and sensitivity in the presence of impurities. Herein, we present an HPLC method based on ion-pair reversed-phase (IP-RP) chromatography to quantify DNA scaffolds. Using IP-RP chromatography, ssDNA products (449 and 1000 nt) prepared by aPCR were separated from impurities and from the double stranded (ds) DNA byproduct. Additionally, both ss and dsDNA were quantified with high accuracy. The method was used to guide the optimization of the production of ssDNA by aPCR, which targeted the maximization of the ratio of ssDNA to dsDNA obtained. Moreover, ssDNA produced from phage infection of E. coli cells was also quantified by IP-RP using commercial ssDNA from the M13mp18 phage as a standard.

引用

页码：22619 / 22624

页数：6

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