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Illumina 测序的原理和应用;Illumina测序流程;Adapter and Library 接头和文库;Illumina测序流程;什么是 flow cell?;1. Single DNA libraries are hybridized to primer lawn and extended by polymerase
;2. Double-stranded molecule is denatured and original template is washed away
;3. New synthesized strand is covalently attached to flow cell surface to form a bridge and extended by polymerase
4. Double-strand bridge is formed
;5. Double-strand bridge is denatured and form
two copies of covalently bound single-stranded templates
6. Bridge amplification cycle repeat
;Multiple bridges are formed
dsDNA bridges are denatured and reverse strands are cleaved
;9. Cleaved reverse strands are washed away and leaving a cluster with forward strands only;Illumina测序流程;Hiseq2500;10. Sequencing primer is hybridized to adapter sequence;11. Only one nucleotide is added every cycle as the 3’ end is blocked;12. Cleave the fluor and free the 3’ end then repeat above steps for next cycle
;13. Sequenced strand is stripped off and the index primer is added for to seq index
;14. Repeat bridge amplification to form reverse strand after index sequencing
15. Sequencing the reverse strands ;高通量测序的应用;高通量测序的应用;
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