An Efficient Guanine O6 Phosphitylation Repair Strategy for High-Quality DNA Library Synthesis via Digital Nucleic Acid Photolithography

Santra Santhosh; Sharon Istvánffy; Omer Sabary; Eitan Yaakobi; Maya Giridhar; Jürgen Behr; Mark Somoza

doi:10.26434/chemrxiv-2025-f706f

An Efficient Guanine O6 Phosphitylation Repair Strategy for High-Quality DNA Library Synthesis via Digital Nucleic Acid Photolithography

Santra Santhosh (First Author), Sharon Istvánffy (Co-Author), Omer Sabary (Co-Author), Eitan Yaakobi (Co-Author), Maya Giridhar (Co-Author), Jürgen Behr (Co-Author), Mark Somoza^* (Last Author)

^*Corresponding author for this work

Transcriptome & Proteome Profiling

Research output: Working paper › Preprint

Abstract

Large-scale de novo nucleic acid synthesis is a powerful tool enabling researchers to better understand and engineer biological systems. Fields ranging from genomics to nucleic acid therapeutics to synthetic biology make use of high-throughput experimental approaches requiring access to large pools or libraries of DNA, RNA, synthetic nucleic acid analogs, non-nucleosidic building blocks, or combinations of these. Large oligonucleotide libraries are synthesized as microarrays and used in situ for surface-based assays or cleaved for off-array applications. Here, using a digital maskless photolithographic approach, we address an important source of error in DNA microarray synthesis, oligonucleotide fragmentation arising from the O6-phosphitylation of guanine during the potentially hundreds of coupling cycles required for complex library synthesis. Introducing a very short debranching step using standard capping reagents suppresses depurination-based fragmentation and greatly enhances synthetic yield.

Original language	American English
DOIs	https://doi.org/10.26434/chemrxiv-2025-f706f
State	Published - 4 Jun 2025

Keywords

Phosphoramidite chemistry
Digital Photolithographic Synthesis
Nucleic acid chemistry

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10.26434/chemrxiv-2025-f706fLicense: CC BY

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EIC Pathfinder 101115134 - DiDAX
Somoza, M. (PI), Sabzalipoor, H. (CoI) & Istvánffy, S. (CoI)
1/11/23 → …
Project: Research

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Efficiency of Digital Photolithographic Synthesis of Large, High-Quality DNA Libraries and Microarrays using a Guanine O⁶ Dephosphitylation Strategy
Santhosh, S. (First Author), Istvánffy, S. (Co-Author), Sabary, O., Yaakobi, E., Giridhar, M. (Co-Author), Behr, J. (Co-Author) & Somoza, M. M. (Last Author), 31 Oct 2025, In: Communications Chemistry. 8, 1, 321.
Research output: Contribution to journal › Article › peer-review

Open Access

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Optimizing Sequence Fidelity in DNA Microarray Synthesis Incorporating Debranching Strategy
Santhosh, S. (Speaker)
3 Sep 2024 → 6 Sep 2024
Activity: Talk or event contribution › Poster presentation

Cite this

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title = "An Efficient Guanine O6 Phosphitylation Repair Strategy for High-Quality DNA Library Synthesis via Digital Nucleic Acid Photolithography",

abstract = "Large-scale de novo nucleic acid synthesis is a powerful tool enabling researchers to better understand and engineer biological systems. Fields ranging from genomics to nucleic acid therapeutics to synthetic biology make use of high-throughput experimental approaches requiring access to large pools or libraries of DNA, RNA, synthetic nucleic acid analogs, non-nucleosidic building blocks, or combinations of these. Large oligonucleotide libraries are synthesized as microarrays and used in situ for surface-based assays or cleaved for off-array applications. Here, using a digital maskless photolithographic approach, we address an important source of error in DNA microarray synthesis, oligonucleotide fragmentation arising from the O6-phosphitylation of guanine during the potentially hundreds of coupling cycles required for complex library synthesis. Introducing a very short debranching step using standard capping reagents suppresses depurination-based fragmentation and greatly enhances synthetic yield.",

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AU - Santhosh, Santra

AU - Istvánffy, Sharon

AU - Sabary , Omer

AU - Yaakobi, Eitan

AU - Giridhar, Maya

AU - Behr, Jürgen

AU - Somoza, Mark

PY - 2025/6/4

Y1 - 2025/6/4

N2 - Large-scale de novo nucleic acid synthesis is a powerful tool enabling researchers to better understand and engineer biological systems. Fields ranging from genomics to nucleic acid therapeutics to synthetic biology make use of high-throughput experimental approaches requiring access to large pools or libraries of DNA, RNA, synthetic nucleic acid analogs, non-nucleosidic building blocks, or combinations of these. Large oligonucleotide libraries are synthesized as microarrays and used in situ for surface-based assays or cleaved for off-array applications. Here, using a digital maskless photolithographic approach, we address an important source of error in DNA microarray synthesis, oligonucleotide fragmentation arising from the O6-phosphitylation of guanine during the potentially hundreds of coupling cycles required for complex library synthesis. Introducing a very short debranching step using standard capping reagents suppresses depurination-based fragmentation and greatly enhances synthetic yield.

AB - Large-scale de novo nucleic acid synthesis is a powerful tool enabling researchers to better understand and engineer biological systems. Fields ranging from genomics to nucleic acid therapeutics to synthetic biology make use of high-throughput experimental approaches requiring access to large pools or libraries of DNA, RNA, synthetic nucleic acid analogs, non-nucleosidic building blocks, or combinations of these. Large oligonucleotide libraries are synthesized as microarrays and used in situ for surface-based assays or cleaved for off-array applications. Here, using a digital maskless photolithographic approach, we address an important source of error in DNA microarray synthesis, oligonucleotide fragmentation arising from the O6-phosphitylation of guanine during the potentially hundreds of coupling cycles required for complex library synthesis. Introducing a very short debranching step using standard capping reagents suppresses depurination-based fragmentation and greatly enhances synthetic yield.

KW - Phosphoramidite chemistry

KW - Digital Photolithographic Synthesis

KW - Nucleic acid chemistry

U2 - 10.26434/chemrxiv-2025-f706f

DO - 10.26434/chemrxiv-2025-f706f

M3 - Preprint

BT - An Efficient Guanine O6 Phosphitylation Repair Strategy for High-Quality DNA Library Synthesis via Digital Nucleic Acid Photolithography

ER -

An Efficient Guanine O6 Phosphitylation Repair Strategy for High-Quality DNA Library Synthesis via Digital Nucleic Acid Photolithography

Abstract

Keywords

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Projects

EIC Pathfinder 101115134 - DiDAX

Research output

Efficiency of Digital Photolithographic Synthesis of Large, High-Quality DNA Libraries and Microarrays using a Guanine O6 Dephosphitylation Strategy

Activities

Optimizing Sequence Fidelity in DNA Microarray Synthesis Incorporating Debranching Strategy

Cite this

Efficiency of Digital Photolithographic Synthesis of Large, High-Quality DNA Libraries and Microarrays using a Guanine O⁶ Dephosphitylation Strategy