Small RNA-seq dataset of wild type and 16C Nicotiana benthamiana leaves sprayed with naked dsRNA using the high-pressure spraying technique

Double-stranded RNA (dsRNA) applications have emerged as promising alternatives to chemical plant pesticides. It has been proposed that the protective effect of dsRNA is mediated by the RNA interference (RNAi) mechanism. Small RNAs (sRNAs) are one of the landmarks of RNAi mechanisms. Two classes of...

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Main Authors: Kübra Çalışır, Gabi Krczal, Veli Vural Uslu
Format: Article
Language:English
Published: Elsevier 2022-12-01
Series:Data in Brief
Subjects:
Online Access:http://www.sciencedirect.com/science/article/pii/S2352340922009106
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author Kübra Çalışır
Gabi Krczal
Veli Vural Uslu
author_facet Kübra Çalışır
Gabi Krczal
Veli Vural Uslu
author_sort Kübra Çalışır
collection DOAJ
description Double-stranded RNA (dsRNA) applications have emerged as promising alternatives to chemical plant pesticides. It has been proposed that the protective effect of dsRNA is mediated by the RNA interference (RNAi) mechanism. Small RNAs (sRNAs) are one of the landmarks of RNAi mechanisms. Two classes of sRNAs appear upon RNAi, triggered by dsRNA: The cleavage products of the dsRNA mapping directly to the dsRNA sequence and the transitive sRNAs mapping to the target transcript outside of the dsRNA sequence. Therefore, the sRNA-seq data obtained from dsRNA-treated plants have been exclusively analysed in the context of the target genes and the outcome has been considered essential to evaluate the underlying mechanism of dsRNA mediated plant protection. Using high-pressure spraying technology (HPST), we have applied a GFP targeting 139bp-long dsRNA on wild type (WT) and GFP expressing (16C) Nicotiana benthamiana plants in biological triplicates. As a control, we applied water with HPST on 16C N. benthamiana. We have acquired sRNA-seq data on the treated and control leaves 5 days post spraying. In this dataset, we have expanded our sRNA-seq analysis from the target GFP transgene sequence to the whole transcriptome of N. benthamiana to provide the community with a resource for the small RNA landscape after high-pressure spraying in 16C and WT samples. Furthermore, we have provided a comparison of sRNA landscape between WT and 16C lines.
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spelling doaj.art-040b85ce4c604137a6eed467836cc0292022-12-22T04:38:02ZengElsevierData in Brief2352-34092022-12-0145108706Small RNA-seq dataset of wild type and 16C Nicotiana benthamiana leaves sprayed with naked dsRNA using the high-pressure spraying techniqueKübra Çalışır0Gabi Krczal1Veli Vural Uslu2Molecular Biology and Genetics Department, Bilkent University, Ankara, TurkeyBioeconomy Department, RLP AgroScience GmbH, Neustadt an der Weinstraße, GermanyBioeconomy Department, RLP AgroScience GmbH, Neustadt an der Weinstraße, Germany; Molecular and Applied Plant Sciences, Center for Organismal Studies, Heidelberg University, Heidelberg, Germany; Corresponding author.Double-stranded RNA (dsRNA) applications have emerged as promising alternatives to chemical plant pesticides. It has been proposed that the protective effect of dsRNA is mediated by the RNA interference (RNAi) mechanism. Small RNAs (sRNAs) are one of the landmarks of RNAi mechanisms. Two classes of sRNAs appear upon RNAi, triggered by dsRNA: The cleavage products of the dsRNA mapping directly to the dsRNA sequence and the transitive sRNAs mapping to the target transcript outside of the dsRNA sequence. Therefore, the sRNA-seq data obtained from dsRNA-treated plants have been exclusively analysed in the context of the target genes and the outcome has been considered essential to evaluate the underlying mechanism of dsRNA mediated plant protection. Using high-pressure spraying technology (HPST), we have applied a GFP targeting 139bp-long dsRNA on wild type (WT) and GFP expressing (16C) Nicotiana benthamiana plants in biological triplicates. As a control, we applied water with HPST on 16C N. benthamiana. We have acquired sRNA-seq data on the treated and control leaves 5 days post spraying. In this dataset, we have expanded our sRNA-seq analysis from the target GFP transgene sequence to the whole transcriptome of N. benthamiana to provide the community with a resource for the small RNA landscape after high-pressure spraying in 16C and WT samples. Furthermore, we have provided a comparison of sRNA landscape between WT and 16C lines.http://www.sciencedirect.com/science/article/pii/S2352340922009106RNAidsRNAsRNA-seqexoRNASIGSPTGS
spellingShingle Kübra Çalışır
Gabi Krczal
Veli Vural Uslu
Small RNA-seq dataset of wild type and 16C Nicotiana benthamiana leaves sprayed with naked dsRNA using the high-pressure spraying technique
Data in Brief
RNAi
dsRNA
sRNA-seq
exoRNA
SIGS
PTGS
title Small RNA-seq dataset of wild type and 16C Nicotiana benthamiana leaves sprayed with naked dsRNA using the high-pressure spraying technique
title_full Small RNA-seq dataset of wild type and 16C Nicotiana benthamiana leaves sprayed with naked dsRNA using the high-pressure spraying technique
title_fullStr Small RNA-seq dataset of wild type and 16C Nicotiana benthamiana leaves sprayed with naked dsRNA using the high-pressure spraying technique
title_full_unstemmed Small RNA-seq dataset of wild type and 16C Nicotiana benthamiana leaves sprayed with naked dsRNA using the high-pressure spraying technique
title_short Small RNA-seq dataset of wild type and 16C Nicotiana benthamiana leaves sprayed with naked dsRNA using the high-pressure spraying technique
title_sort small rna seq dataset of wild type and 16c nicotiana benthamiana leaves sprayed with naked dsrna using the high pressure spraying technique
topic RNAi
dsRNA
sRNA-seq
exoRNA
SIGS
PTGS
url http://www.sciencedirect.com/science/article/pii/S2352340922009106
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