Julia Salzman scite author profile

The vast landscape of RNA-protein interactions at the heart of post-transcriptional regulation remains largely unexplored. Indeed it is likely that, even in yeast, a substantial fraction of the regulatory RNA-binding proteins (RBPs) remain to be discovered. Systematic experimental methods can play a key role in discovering these RBPs - most of the known yeast RBPs lack RNA-binding domains that might enable this activity to be predicted. We describe here a proteome-wide approach to identify RNA-protein interactions based on in vitro binding of RNA samples to yeast protein microarrays that represent over 80% of the yeast proteome. We used this procedure to screen for novel RBPs and RNA-protein interactions. A complementary mass spectrometry technique also identified proteins that associate with yeast mRNAs. Both the protein microarray and mass spectrometry methods successfully identify previously annotated RBPs, suggesting that other proteins identified in these assays might be novel RBPs. Of 35 putative novel RBPs identified by either or both of these methods, 12, including 75% of the eight most highly-ranked candidates, reproducibly associated with specific cellular RNAs. Surprisingly, most of the 12 newly discovered RBPs were enzymes. Functional characteristics of the RNA targets of some of the novel RBPs suggest coordinated post-transcriptional regulation of subunits of protein complexes and a possible link between mRNA trafficking and vesicle transport. Our results suggest that many more RBPs still remain to be identified and provide a set of candidates for further investigation.

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The Tabula Sapiens: A multiple-organ, single-cell transcriptomic atlas of humans

Jones¹,

Karkanias²,

Bulthaup³

et al. 2022

Science

468

145

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Molecular characterization of cell types using single-cell transcriptome sequencing is revolutionizing cell biology and enabling new insights into the physiology of human organs. We created a human reference atlas comprising nearly 500,000 cells from 24 different tissues and organs, many from the same donor. This atlas enabled molecular characterization of more than 400 cell types, their distribution across tissues, and tissue-specific variation in gene expression. Using multiple tissues from a single donor enabled identification of the clonal distribution of T cells between tissues, identification of the tissue-specific mutation rate in B cells, and analysis of the cell cycle state and proliferative potential of shared cell types across tissues. Cell type–specific RNA splicing was discovered and analyzed across tissues within an individual.

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Extensive site-directed mutagenesis reveals interconnected functional units in the alkaline phosphatase active site

Sunden

Peck

Salzman

et al. 2015

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Enzymes enable life by accelerating reaction rates to biological timescales. Conventional studies have focused on identifying the residues that have a direct involvement in an enzymatic reaction, but these so-called ‘catalytic residues’ are embedded in extensive interaction networks. Although fundamental to our understanding of enzyme function, evolution, and engineering, the properties of these networks have yet to be quantitatively and systematically explored. We dissected an interaction network of five residues in the active site of Escherichia coli alkaline phosphatase. Analysis of the complex catalytic interdependence of specific residues identified three energetically independent but structurally interconnected functional units with distinct modes of cooperativity. From an evolutionary perspective, this network is orders of magnitude more probable to arise than a fully cooperative network. From a functional perspective, new catalytic insights emerge. Further, such comprehensive energetic characterization will be necessary to benchmark the algorithms required to rationally engineer highly efficient enzymes.DOI: http://dx.doi.org/10.7554/eLife.06181.001

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The SpliZ generalizes “Percent Spliced In” to reveal regulated splicing at single-cell resolution

Olivieri¹,

Dehghannasiri²,

Salzman

2020

Preprint

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To date, the field of single-cell genomics has viewed robust splicing analysis as completely out of reach in droplet-based platforms, preventing biological discovery of single-cell regulated splicing. Here, we introduce a novel, robust, and computationally efficient statistical method, the Splicing Z Score (SZS), to detect differential alternative splicing in single cell RNA-Seq technologies including 10x Chromium. We applied the SZS to primary human cells to discover new regulated, cell type-specific splicing patterns. Illustrating the power of the SZS method, splicing of a small set of genes has high predictive power for tissue compartment in the human lung, and the SZS identifies un-annotated, conserved splicing regulation in the human spermatogenesis. The SZS is a method that can rapidly identify regulated splicing events from single cell data and prioritize genes predicted to have functionally significant splicing programs.

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Julia Salzman

Proteome-Wide Search Reveals Unexpected RNA-Binding Proteins in Saccharomyces cerevisiae

The Tabula Sapiens: A multiple-organ, single-cell transcriptomic atlas of humans

Extensive site-directed mutagenesis reveals interconnected functional units in the alkaline phosphatase active site

The SpliZ generalizes “Percent Spliced In” to reveal regulated splicing at single-cell resolution

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