varieties, transgenic or knockout lines able to maintain their green color longer than wild-type plants. In these plants, long-lasting leaf coloration is correlated to durable chlorophyll accumulation compared to wild-type plants or standard varieties, and it is often associated with delayed senescence 52. In Arabidopsis, senescence mechanisms induce the expression of ORESARA1 (ORE1) and ORE1 SISTER1 (ORS1) genes. ORE1 activates program cell death and ORS1 participates to salt-induced senescence; the corresponding knockout mutant plants display a stay-green phenotype and delayed senescence 19,20,22,26. Conversely, the disruption of VND-INTERACTING2 (VNI2) and JUNGBRUNNEN1 (JUB1)-which also encode for two NAC proteins-causes early senescence while their overexpression induces a stay-green phenotype 24,53. Recently, it was demonstrated that transgenic tomato lines, with reduced accumulation of SlNAP2 messenger (Solanum lycopersicum NAC-like, activated by Apetala3/ Pistillata), display a stay-green phenotype even upon ABA (abscisic acid) application 33. In this manuscript, we describe the role of Solyc12g036480, which encodes a NAC transcription factor able to modulate leaf senescence in tomato. We demonstrate that Solyc12g036480 downregulation, achieved via Virusinduced gene silencing (VIGS), confers longer life span and delayed overall senescence in tomato plants; for this reason we named this gene HḖBĒ (HEB) after the Greek youth goddess. Results and discussion HEB expression analyses. The tomato NAC TFs family counts 101 members and only few of them have been functionally characterized. As yet, tomato NAC proteins have been described as involved in defense responses, stomata opening and closure, drought tolerance, flower-boundary morphogenesis, leaf senescence and fruit ripening 33,54-57. Among these 101 NAC members, we have selected Solyc12g036480/HEB for a deeper characterization. According to the transcriptome data collection of the Tomato Genome Consortium, HEB is equally transcribed in leaves and roots, but from the experimental data of Huang and Schiefelbein, HEB messenger is not detected in roots 58,59. In order to define temporally and spatially HEB expression pattern, quantitative Real-Time PCRs (qRT-PCRs) were performed. Expression analyses were carried out using organs dissected by Micro-tom plants; UBIQUITIN 3 (UBI3) and ELONGATION FACTOR 1α (EF1α) were used as reference genes 60. HEB transcript was found in young and old leaves and in young floral buds, but its mRNA is barely detected in roots, stem, mature green and red ripe fruits [developmental stages as described in 61 (Fig. 1)].
