Analyzing Flowering Time Genes in Arabidopsis

Total RNA was isolated from 9-day-old seedlings using Plant RNA Purification Reagent (Invitrogen, USA). The total extracted RNA was pretreated with DNase I (NEB, USA) to eliminate possible DNA contamination, and subsequently subjected to complementary DNA synthesis using the First Strand cDNA Synthesis Kit (Roche Applied Science, USA). To measure the transcript levels of flowering time genes, quantitative real-time RT-PCR (qPCR) was carried out using the Green I Master Mix (Roche Applied Science, USA) with gene-specific primers (Supplementary Table S1). Two reference genes (AT1G13320/AT2G28390) that are stably expressed (Hong et al., 2010 (link)) were used for quantification. All reactions were performed with two biological replicates and three technical replicates. Determination of mature miR156 levels was done by miRNA northern hybridization analysis, as described previously (Lee et al., 2010 (link)). For histochemical GUS analysis, transgenic plants expressing MIR156::GUS were generated. The promoter region (approximately 2 kb) of MIR156b was amplified by PCR (Supplementary Table S1), and then cloned into the pBI101 vector harboring a GUS reporter gene. The resulting MIR156::GUS construct was introduced into wild-type and double mutant (agl15-3 agl18-1 and agl15-4 agl18-1) plants using a floral dip method (Clough and Bent, 1998 (link)).

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Serivichyaswat P., Ryu H.S., Kim W., Kim S., Chung K.S., Kim J.J, & Ahn J.H. (2015). Expression of the Floral Repressor miRNA156 is Positively Regulated by the AGAMOUS-like Proteins AGL15 and AGL18. Molecules and Cells, 38(3), 259-266.

Publication 2015

Plant RNA Purification Reagent DNase I First Strand cDNA Synthesis Kit Green I Master Mix

Bent Biological Cdna Dna contamination Dna synthesis Dnase i Genes Hybridization Mirna Plant rna Plants Primers Quantitative real time pcr Reporter gene Seedlings Synthesis Transgenic plants Vector

Corresponding Organization : Korea University

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Variable analysis

independent variables

Genotype (wild-type, agl15-3 agl18-1, agl15-4 agl18-1)

dependent variables

Transcript levels of flowering time genes
Mature miR156 levels
GUS reporter gene expression

control variables

Total RNA from 9-day-old seedlings
DNase I treatment to eliminate DNA contamination
Two reference genes (AT1G13320/AT2G28390) for qPCR quantification
Two biological replicates and three technical replicates for qPCR

positive controls

None specified

negative controls

None specified

Annotations

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