Literature DB >> 29300409

Concentrating and labeling genomic DNA in a nanofluidic array.

Rodolphe Marie1, Jonas N Pedersen, Kalim U Mir, Brian Bilenberg, Anders Kristensen.   

Abstract

Nucleotide incorporation by DNA polymerase forms the basis of DNA sequencing-by-synthesis. In current platforms, either the single-stranded DNA or the enzyme is immobilized on a solid surface to locate the incorporation of individual nucleotides in space and/or time. Solid-phase reactions may, however, hinder the polymerase activity. We demonstrate a device and a protocol for the enzymatic labeling of genomic DNA arranged in a dense array of single molecules without attaching the enzyme or the DNA to a surface. DNA molecules accumulate in a dense array of pits embedded within a nanoslit due to entropic trapping. We then perform ϕ29 polymerase extension from single-strand nicks created on the trapped molecules to incorporate fluorescent nucleotides into the DNA. The array of entropic traps can be loaded with λ-DNA molecules to more than 90% of capacity at a flow rate of 10 pL min-1. The final concentration can reach up to 100 μg mL-1, and the DNA is eluted from the array by increasing the flow rate. The device may be an important preparative module for carrying out enzymatic processing on DNA extracted from single-cells in a microfluidic chip.

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Year:  2018        PMID: 29300409     DOI: 10.1039/c7nr06016e

Source DB:  PubMed          Journal:  Nanoscale        ISSN: 2040-3364            Impact factor:   7.790


  2 in total

1.  Microfluidic long DNA sample preparation from cells.

Authors:  Paridhi Agrawal; Kevin D Dorfman
Journal:  Lab Chip       Date:  2019-01-15       Impact factor: 6.799

2.  A Complete Protocol for Rapid and Low-Cost Fabrication of Polymer Microfluidic Chips Containing Three-Dimensional Microstructures Used in Point-of-Care Devices.

Authors:  Trieu Nguyen; Aaydha Chidambara Vinayaka; Dang Duong Bang; Anders Wolff
Journal:  Micromachines (Basel)       Date:  2019-09-19       Impact factor: 2.891

  2 in total

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