PI3K-related kinases (PIKKs) are large Serine/Threonine (Ser/Thr)-protein kinases central to the regulation of many fundamental cellular processes. PIKK family member SMG1 orchestrates progression of an RNA quality control pathway, termed nonsense-mediated mRNA decay (NMD), by phosphorylating the NMD factor UPF1. Phosphorylation of UPF1 occurs in its unstructured N- and C-terminal regions at Serine/Threonine-Glutamine (SQ) motifs. How SMG1 and other PIKKs specifically recognize SQ motifs has remained unclear. Here, we present a cryo-electron microscopy (cryo-EM) reconstruction of a human SMG1-8-9 kinase complex bound to a UPF1 phosphorylation site at an overall resolution of 2.9 Å. This structure provides the first snapshot of a human PIKK with a substrate-bound active site. Together with biochemical assays, it rationalizes how SMG1 and perhaps other PIKKs specifically phosphorylate Ser/Thr-containing motifs with a glutamine residue at position +1 and a hydrophobic residue at position -1, thus elucidating the molecular basis for phosphorylation site recognition.
Keywords: Cryo-EM; PIKK; RNA quality control; human; molecular biophysics; nonsense-mediated mRNA decay; phosphorylation; structural biology.
The instructions for producing proteins in the cell are copied from DNA to molecules known as messenger RNA. If there is an error in the messenger RNA, this causes incorrect proteins to be produced that could potentially kill the cell. Cells have a special detection system that spots and removes any messenger RNA molecules that contain errors, which would result in the protein produced being too short. For this error-detecting system to work, a protein called UPF1 must be modified by an enzyme called SMG1. This enzyme only binds to and modifies the UPF1 protein at sites that contain a specific pattern of amino acids – the building blocks that proteins are made from. However, it remained unclear how SMG1 recognizes this pattern and interacts with UPF1. Now, Langer et al. have used a technique known as cryo-electron microscopy to image human SMG1 bound to a segment of UPF1. These images were then used to generate the three-dimensional structure of how the two proteins interact. This high-resolution structure showed that protein building blocks called leucine, serine and glutamine are the recognized pattern of amino acids. To further understand the role of the amino acids, Langer et al. replaced them one-by-one with different amino acids to see how each affected the interaction between the two proteins. This revealed that SMG1 preferred leucine at the beginning of the recognized pattern and glutamine at the end when binding to UPF1. SMG1 is member of an important group of enzymes that are involved in various error detecting systems. This is the first time that a protein from this family has been imaged together with its target and these findings may also be relevant to other enzymes in this family. Furthermore, the approach used to determine the structure of SMG1 and the structural information itself could also be used in drug design to improve the accuracy with which drugs identify their targets.
© 2020, Langer et al.