Abstract

To accommodate fluctuating nutrient levels in the soil, plants modulate their metabolism and root development via signaling mechanisms that rapidly reprogram the plant transcriptome. In the case of nitrate, over 1,000 genes are induced or repressed within minutes of nitrate exposure. To identify cis-regulatory elements that mediate these responses, an enhancer screen was performed in transgenic Arabidopsis (Arabidopsis thaliana) plants. A 1.8-kb promoter fragment from the nitrate reductase gene NIA1 was identified that acts as a nitrate enhancer when fused to a 35S minimal promoter. Enhancer activity was localized to a 180-bp fragment, and this activity could be enhanced by the addition of a 131-bp fragment from the nitrite reductase promoter. A promoter construct containing the 180- and 131-bp fragments was also induced by nitrite and repressed by ammonium, indicating that it was responsive to multiple nitrogen signals. To identify specific regulatory elements within the 180-bp NIA1 fragment, a transient expression system using agroinfiltration of Nicotiana benthamiana was developed. Deletion analysis identified three elements corresponding to predicted binding motifs for homeodomain/E-box, Myb, and Alfin1 transcription factors. A fully active promoter showing nitrate and nitrite enhancer activity equivalent to that of the wild-type 180-bp fragment could be built from these three elements if the spacing between the homeodomain/E-box and Myb-Alfin1 sites was equivalent to that of the native promoter. These findings were validated in transgenic Arabidopsis plants and identify a cis-regulatory module containing three elements that comprise a nitrate enhancer in the NIA1 promoter.

Highlights

  • To accommodate fluctuating nutrient levels in the soil, plants modulate their metabolism and root development via signaling mechanisms that rapidly reprogram the plant transcriptome

  • Our search for nitrate enhancer elements (NEEs) began with a screen for enhancer fragments from the nitrate reductase gene NIA1 (At1g77760)

  • Out of four NIA1 fragments tested, only one showed nitrate enhancer activity (Supplemental Fig. S1)

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Summary

Introduction

To accommodate fluctuating nutrient levels in the soil, plants modulate their metabolism and root development via signaling mechanisms that rapidly reprogram the plant transcriptome. A fully active promoter showing nitrate and nitrite enhancer activity equivalent to that of the wild-type 180-bp fragment could be built from these three elements if the spacing between the homeodomain/E-box and Myb-Alfin sites was equivalent to that of the native promoter These findings were validated in transgenic Arabidopsis plants and identify a cisregulatory module containing three elements that comprise a nitrate enhancer in the NIA1 promoter. 1,500 genes are rapidly induced or repressed by nitrate and that the processes of pentose phosphate oxidation, glycolysis, trehalose synthesis, nitrogen, and amino acid metabolism are most affected (Wang et al, 2003, 2004, 2007; Scheible et al, 2004; Gutierrez et al, 2007) These rapid transcriptome responses provide the basis for the longer-term responses that direct root growth, development, and architecture, root-to-shoot ratios, and germination rates (Forde, 2002; Alboresi et al, 2005; Filleur et al, 2005; Forde and Walch-Liu, 2009). CIPK23 phosphorylates the nitrate transporter NRT1.1 (CHL1; Tsay et al, 1993), which has been shown to act as a nitrate regulator/ sensor (Ho et al, 2009; Wang et al, 2009; Krouk et al, 2010)

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