摘要
The Human Genome Project opened an era of(epi)genomic research,and also provided a platform for the development of new sequencing technologies.During and after the project,several sequencing technologies continue to dominate nucleic acid sequencing markets.Currently,Illumina(short-read),PacBio(long-read),and Oxford Nanopore(longread)are the most popular sequencing technologies.Unlike PacBio or the popular short-read sequencers before it,which,as examples of the second or so-called Next-Generation Sequencing platforms,need to synthesize when sequencing,nanopore technology directly sequences native DNA and RNA molecules.Nanopore sequencing,therefore,avoids converting mRNA into cDNA molecules,which not only allows for the sequencing of extremely long native DNA and full-length RNA molecules but also document modifications that have been made to those native DNA or RNA bases.In this review on direct DNA sequencing and direct RNA sequencing using Oxford Nanopore technology,we focus on their development and application achievements,discussing their challenges and future perspective.We also address the problems researchers may encounter applying these approaches in their research topics,and how to resolve them.
基金
supported by the Key-Areas Research and Development Program of Guangdong Province(2020B020220004)
the Youth Innovation Promotion Association,Chinese Academy of Sciences(2017399)
the Science and Technology Program of Guangzhou(202002030097)
the Hong Kong Research Grants Council Area of Excellence Scheme(AoE/M-403/16),the ECS(27204518)
TRS of the HKSAR government(T21-705/20-N).
