Functional profiling of the male gametophyte-specific promoter fragment ofArabidopsis PIRL6gene and prediction ofcis-regulatory elements

Abstract

AbstractGametophyte-specific promoters drive the expression of genes in male and/or female gametophytes. These have applications in breeding experiments, gene function identification, developmental biology-related studies, and off-lately in genome editing also. ThePlant Intracellular Ras-group Leucine-Rich-Repeat6 (PIRL6) gene is known to be necessary for male and female gametogenesis. Using theGUS-based deletion analysis, we have identified thePIRL6promoter length that is essential for exclusive expression in the male gametophyte ofArabidopsis thaliana.We studied the strength of various lengths ofPIRL6promoters in different tissues, by GUS expression quantification. The male-gametophyte-specific promoter segment (PA1) exhibited stronger expression in mature anthers than the younger ones. We identified 50 other genes that co-expressed withPIRL6inArabidopsisusing the Expression Angler tool. Gene ontology (GO) analysis shows that these 51 co-expressing genes were predominantly involved in cell differentiation. By comparing the promoter sequences of these 51 genes, the presence of three over-represented known motifs, POLLEN1LELAT52, ACGTATERD1 and CIACADIANLELHC was identified. We could also predict the presence of three novelcis-regulatory elements in the co-expressing gene network using the MEME suite tool. Additionally, we confirmed the functionality of the ABRE and P-box elements present inPIRL6promoter using the tobacco leaf transient assay. Thus, we cloned and functionally confirmed the promoter region ofPIRL6required for male gametophyte-specific expression, compared this promoter with those of 50 other co-expressed genes and predicted their functions, and analyzed theircisregulatory regions and predicted three novel motifs also.Key messageA pollen-specific promoter fragment ofPIRL6was functionally characterized usingGUS-based deletion analysis. Fifty other co-expressed genes were compared and novelcis-regulatory elements were predicted. Two hormone-responsive elements in thePIRL6promoter were found to influence theGUSexpression. PA1 promoter can be used in experiments that require male gametophyte-specific expression of genes.