Pathogen-induced accumulation of the immune hormone SA leads to dramatic reprogramming of cellular gene expression to prioritise immune response activation over other cellular household processes. SA triggers massive gene expression changes through its nuclear receptor protein, NPR1, a potent gene activator. SA-induced modification of NPR1 by the small post-translational modifier, ubiquitin, regulates its activity and lifetime, thereby functioning as an instruction manual for onset of immunity. Importantly, proteins such as NPR1 are modified by chains of interlinked ubiquitin of different structural topologies, but the biological effects of these chain topologies remain poorly understood. We investigated how SA orchestrates ubiquitin-mediated activation of NPR1. Surprisingly, we discovered that SA-induced NPR1 is subject to a relay of three different ubiquitin ligases that each have distinct effects on its activity. First, a modular Cullin3-RING Ligase (CRL3) modifies NPR1 with a short ubiquitin chain of a specific topology. This short ubiquitin chain is a platform for the recruitment of additional transcriptional regulators that together with NPR1 attract the necessary machinery for activation of immune genes. Unlike CRL3, the subsequent UBE4 ubiquitin ligase deactivates NPR1 by extending its ubiquitin chains with a different topology. This results in chains of mixed topologies that target NPR1 for degradation by the proteasome. Despite having already been recruited to the proteasome, NPR1 is subject to further ubiquitination by the proteasome-associated HECT-type ligases, UPL3 and UPL4. This ‘eleventh hour’ modification prevents stalling of the proteasome during the degradation of NPR1. Subsequently, we discovered that other gene activators are also regulates by ubiquitin ligase relays, suggesting they are a universal mechanism for regulating the lifetimes and activities of proteasome-targeted substrates.
So why is NPR1 subject to such complicated control by a relay of multiple different ubiquitin ligases? We hypothesised that NPR1 activity if tightly controlled by ubiquitin signalling, because its dysregulation leads to pathological conditions, including autoimmunity. Could it be NPR1 is such a potent gene activator that its uncontrolled activity risks genome instability caused by excessive demand for gene expression? In support of this notion, we discovered that mutants with enhanced NPR1 activity are sensitive to DNA damage and that NPR1 physically interacts with a number of DNA repair proteins. Thus, the project now explores if dynamic ubiquitin signalling curbs NPR1 activity to avoid genomic instability associated with excessive demands for gene expression.
To further explore how SA-induced ubiquitin signalling orchestrates activation of immunity, we established a proteomics pipeline for detection of protein ubiquitination. This has allowed us to define the immune-induced ubiquitin chain topology landscape and observe direct links between specific ubiquitin topologies and cellular processes. For example, we discovered that activation of immunity induces novel changes in the ubiquitination of histones that are key DNA packaging proteins for stabilisation of the genetic code. Our findings suggest that histone ubiquitination at previously unrecognised sites is critical for the activation of immune responses.
