In yeast, H3K4 methylation is carried out by the Set1 complex (Set1C). H2B ubiquitylation directly stimulates nucleosomal H3K4 methylation by Set1C. A minimal set of protein subunits and interactions are required for this process that includes Set1, Spp1 and several conserved Set1C subunits. This study examines how Set1C subunits sense H2B ubiquitylation and how they activate the catalytic function of Set1C to methylate nucleosomal H3K4. The study provides evidence that all essential components required for H2B ubiquitylation-dependent H3K4 methylation are interconnected within the active site of Set1C and are subjected to conformational changes upon sensing H2B ubiquitylation. It indicates that physical interaction of the N-terminus of Set1 with Swd1 located within the catalytic core enables Set1C to methylate nucleosomal H3K4 in the absence of Spp1. The study explains why ‘full-length’ Set1-containing Set1C is able to methylate H3K4 in the absence of Spp1.

A long-standing question is why retroviruses package 2 copies of RNA genomes when each infection event generates only 1 provirus. Recombination increases genetic diversity and generates HIV-1 variants that are resistant to antivirals or can escape immune responses. It also plays an important role in shaping the HIV epidemic as evidenced by multiple circulating recombinant forms. Although the role of recombination in generating genetic diversity has been clear, it was unknown whether this process is required for efficient HIV-1 replication. This study demonstrates that when recombination is inhibited in a part of the HIV-1 genome, viral titers decreased, and proviruses had deletions in regions where recombination was blocked. These results illustrate that recombination is a mechanism required to maintain HIV-1 genome integrity and provide insights into the benefit of packaging 2 seemingly redundant RNA genomes: it allows recombination to take place to salvage genetic information.

This article reports important new understandings in an enzyme/process used by researchers world wide: in vitro transcription by T7 RNA polymerase. While this is the system of choice for RNA synthesis, it is well known to have limitations, a primary one being “nontemplated” 3’ extensions. This is important to the burgeoning field of RNA therapeutics, but plagues researchers throughout basic science and nanotechnology, as well. Reports over two decades have been conflicting and limited in scope. This article brings a new tool, RNA-Seq, to this problem. The RNA-Seq data drive hypotheses that are tested by more conventional tools, but they also indicate a heterogeneity in this process not previously appreciated. This work will prompt development of approaches for mitigating/eliminating this undesired process. While the practical aspects of this work will be interesting to a very wide audience, the results are also of interest to those studying mechanistic elements of transcription.