Journal Articles

Conditional lifetime expectancy function [Statistics]

The conditional lifetime expectancy function (LEF) is the expected lifetime of a subject given survival past a certain time point and the values of a set of explanatory variables. This function is attractive to researchers because it summarizes the entire residual life distribution and has an easy interpretation compared with...
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Sahelian regreening and degradation [Sustainability Science]

Over many decades our understanding of the impacts of intermittent drought in water-limited environments like the West African Sahel has been influenced by a narrative of overgrazing and human-induced desertification. The desertification narrative has persisted in both scientific and popular conception, such that recent regional-scale recovery (“regreening”) and local success...
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Synthetic dosage lethality and cancer survival [Systems Biology]

Synthetic dosage lethality (SDL) denotes a genetic interaction between two genes whereby the underexpression of gene A combined with the overexpression of gene B is lethal. SDLs offer a promising way to kill cancer cells by inhibiting the activity of SDL partners of activated oncogenes in tumors, which are often...
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Correction for Futrell et al., Large-scale evidence of dependency length minimization in 37 languages [Correction]

PSYCHOLOGICAL AND COGNITIVE SCIENCES Correction for “Large-scale evidence of dependency length minimization in 37 languages,” by Richard Futrell, Kyle Mahowald, and Edward Gibson, which appeared in issue 33, August 18, 2015, of Proc Natl Acad Sci USA (112:10336–10341; first published August 3, 2015; 10.1073/pnas.1502134112). The authors note that Figs. 2...
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Correction for Lee et al., The opportunistic marine pathogen Vibrio parahaemolyticus becomes virulent by acquiring a plasmid that expresses a deadly toxin [Correction]

MICROBIOLOGY Correction for “The opportunistic marine pathogen Vibrio parahaemolyticus becomes virulent by acquiring a plasmid that expresses a deadly toxin,” by Chung-Te Lee, I-Tung Chen, Yi-Ting Yang, Tzu-Ping Ko, Yun-Tzu Huang, Jiun-Yan Huang, Ming-Fen Huang, Shin-Jen Lin, Chien-Yu Chen, Shih-Shuen Lin, Donald V. Lightner, Han-Ching Wang, Andrew H.-J. Wang, Hao-Ching...
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Correction for Liu et al., Activation of Big Grain1 significantly improves grain size by regulating auxin transport in rice [Correction]

PLANT BIOLOGY Correction for “Activation of Big Grain1 significantly improves grain size by regulating auxin transport in rice,” by Linchuan Liu, Hongning Tong, Yunhua Xiao, Ronghui Che, Fan Xu, Bin Hu, Chengzhen Liang, Jinfang Chu, Jiayang Li, and Chengcai Chu, which appeared in issue 35, September 1, 2015, of Proc...
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Correction for Sadanandom et al., SUMOylation of phytochrome-B negatively regulates light-induced signaling in Arabidopsis thaliana [SI Correction]

PLANT BIOLOGY Correction for “SUMOylation of phytochrome-B negatively regulates light-induced signaling in Arabidopsis thaliana,” by Ari Sadanandom, Éva Ádám, Beatriz Orosa, András Viczián, Cornelia Klose, Cunjin Zhang, Eve-Marie Josse, László Kozma-Bognár, and Ferenc Nagy, which appeared in issue 35, September 1, 2015, of Proc Natl Acad Sci USA (112:11108–11113; first...
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In This Issue [This Week in PNAS]

Mercury and marine mammals Northern elephant seals accumulate MeHg from their prey in the North Pacific. Image courtesy of James Harvey (Moss Landing Marine Laboratories, Moss Landing, CA). Methylmercury (MeHg) is a neurotoxin that accumulates in marine food chains, posing a threat to environmental and human health. High Hg concentrations...
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Unusual oxacycles in the orthosomycin antibiotics [Biochemistry]

Bacteria, fungi, and plants produce an arsenal of complex biomolecules through which they interact and compete with neighbor organisms (1). The machinery that builds these molecules is replete with iron(II)- and 2-(oxo)glutarate-dependent (Fe/2OG) oxygenases, enzymes that catalyze hydroxylation, halogenation, desaturation, ring-closure, ring-expansion, and stereoinversion reactions on pathways to important natural-product...
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Wheat gene for all seasons [Genetics]

Diverse seasonal flowering behaviors drive global adaption of bread wheat (Triticum aestivum), the major crop grown in temperate zones worldwide. Many wheats are sown in autumn and flower only after experiencing the prolonged cold of winter (vernalization). By delaying flowering until spring, the requirement for vernalization minimizes the risk that...
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Cellular factors and herpesviral latent infection [Microbiology]

The herpesviruses are characterized by their ability to undergo a productive infection upon infection of the host organism and then spread to establish a latent infection where they persist in the host. Later, under conditions of stress or other environmental stimuli, they reactivate to undergo a productive infection and spread...
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Time has come for offshore wind power in the US [Opinion]

Offshore wind turbines have been successfully deployed in Europe since 1991, providing thousands of megawatts of clean energy for multiple nations. Ten years ago, it seemed that the United States would follow suit: The US Energy Policy Act of 2005 directed the Department of the Interior (DOI) to establish an...
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Interolog interfaces in protein–protein docking

ABSTRACT

Proteins are essential elements of biological systems, and their function typically relies on their ability to successfully bind to specific partners. Recently, an emphasis of study into protein interactions has been on hot spots, or residues in the binding interface that make a significant contribution to the binding energetics. In this study, we investigate how conservation of hot spots can be used to guide docking prediction. We show that the use of evolutionary data combined with hot spot prediction highlights near-native structures across a range of benchmark examples. Our approach explores various strategies for using hot spots and evolutionary data to score protein complexes, using both absolute and chemical definitions of conservation along with refinements to these strategies that look at windowed conservation and filtering to ensure a minimum number of hot spots in each binding partner. Finally, structure-based models of orthologs were generated for comparison with sequence-based scoring. Using two data sets of 22 and 85 examples, a high rate of top 10 and top 1 predictions are observed, with up to 82% of examples returning a top 10 hit and 35% returning top 1 hit depending on the data set and strategy applied; upon inclusion of the native structure among the decoys, up to 55% of examples yielded a top 1 hit. The 20 common examples between data sets show that more carefully curated interolog data yields better predictions, particularly in achieving top 1 hits. Proteins 2015; 83:1940–1946. © 2015 The Authors. Proteins: Structure, Function, and Bioinformatics Published by Wiley Periodicals, Inc.

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Crystal structure of the Mycobacterium tuberculosis transcriptional regulator Rv0302

Protein Science - Tue, 09/29/2015 - 11:01
Abstract

Mycobacterium tuberculosis is a pathogenic bacterial species, which is neither Gram positive nor Gram negative. It has a unique cell wall, making it difficult to kill and conferring resistance to antibiotics that disrupt cell wall biosynthesis. Thus, the mycobacterial cell wall is critical to the virulence of these pathogens. Recent work shows that the mycobacterial membrane protein large (MmpL) family of transporters contributes to cell wall biosynthesis by exporting fatty acids and lipidic elements of the cell wall. The expression of the Mycobacterium tuberculosis MmpL proteins is controlled by a complicated regulatory network system. Here we report crystallographic structures of two forms of the TetR-family transcriptional regulator Rv0302, which participates in regulating the expression of MmpL proteins. The structures reveal a dimeric, two-domain molecule with architecture consistent with the TetR family of regulators. Comparison of the two Rv0302 crystal structures suggests that the conformational changes leading to derepression may be due to a rigid body rotational motion within the dimer interface of the regulator. Using fluorescence polarization and electrophoretic mobility shift assays, we demonstrate the recognition of promoter and intragenic regions of multiple mmpL genes by this protein. In addition, our isothermal titration calorimetry and electrophoretic mobility shift experiments indicate that fatty acids may be the natural ligand of this regulator. Taken together, these experiments provide new perspectives on the regulation of the MmpL family of transporters.

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Modulation of HIV protease flexibility by the T80N mutation

ABSTRACT

The flexibility of HIV protease (HIVp) plays a critical role in enabling enzymatic activity and is required for substrate access to the active site. While the importance of flexibility in the flaps that cover the active site is well known, flexibility in other parts of the enzyme is also critical for function. One key region is a loop containing Thr 80, which forms the walls of the active site. Although not situated within the active site, amino acid Thr80 is absolutely conserved. The mutation T80N preserves the structure of the enzyme but catalytic activity is completely lost. To investigate the potential influence of the T80N mutation on HIVp flexibility, wide-angle X-ray scattering (WAXS) data was measured for a series of HIVp variants. Starting with a calculated WAXS pattern from a rigid atomic model, the modulations in the intensity distribution caused by structural fluctuations in the protein were predicted by simple analytic methods and compared with the experimental data. An analysis of T80N WAXS data shows that this variant is significantly more rigid than the WT across all length scales. The effects of this single point mutation extend throughout the protein, to alter the mobility of amino acids in the enzymatic core. These results support the contentions that significant protein flexibility extends throughout HIVp and is critical to catalytic function. Proteins 2015; 83:1929–1939. © 2014 Wiley Periodicals, Inc.

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Global analysis of RNA cleavage by 5'-hydroxyl RNA sequencing

Nucleic Acids Research - Tue, 09/29/2015 - 01:41

RNA cleavage by some endoribonucleases and self-cleaving ribozymes produces RNA fragments with 5'-hydroxyl (5'-OH) and 2',3'-cyclic phosphate termini. To identify 5'-OH RNA fragments produced by these cleavage events, we exploited the unique ligation mechanism of Escherichia coli RtcB RNA ligase to attach an oligonucleotide linker to RNAs with 5'-OH termini, followed by steps for library construction and analysis by massively parallel DNA sequencing. We applied the method to RNA from budding yeast and captured known 5'-OH fragments produced by tRNA Splicing Endonuclease (SEN) during processing of intron-containing pre-tRNAs and by Ire1 cleavage of HAC1 mRNA following induction of the unfolded protein response (UPR). We identified numerous novel 5'-OH fragments derived from mRNAs: some 5'-OH mRNA fragments were derived from single, localized cleavages, while others were likely produced by multiple, distributed cleavages. Many 5'-OH fragments derived from mRNAs were produced upstream of codons for highly electrostatic peptides, suggesting that the fragments may be generated by co-translational mRNA decay. Several 5'-OH RNA fragments accumulated during the induction of the UPR, some of which share a common sequence motif that may direct cleavage of these mRNAs. This method enables specific capture of 5'-OH termini and complements existing methods for identifying RNAs with 2',3'-cyclic phosphate termini.

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Tailor: a computational framework for detecting non-templated tailing of small silencing RNAs

Nucleic Acids Research - Tue, 09/29/2015 - 01:41

Small silencing RNAs, including microRNAs, endogenous small interfering RNAs (endo-siRNAs) and Piwi-interacting RNAs (piRNAs), have been shown to play important roles in fine-tuning gene expression, defending virus and controlling transposons. Loss of small silencing RNAs or components in their pathways often leads to severe developmental defects, including lethality and sterility. Recently, non-templated addition of nucleotides to the 3' end, namely tailing, was found to associate with the processing and stability of small silencing RNAs. Next Generation Sequencing has made it possible to detect such modifications at nucleotide resolution in an unprecedented throughput. Unfortunately, detecting such events from millions of short reads confounded by sequencing errors and RNA editing is still a tricky problem. Here, we developed a computational framework, Tailor, driven by an efficient and accurate aligner specifically designed for capturing the tailing events directly from the alignments without extensive post-processing. The performance of Tailor was fully tested and compared favorably with other general-purpose aligners using both simulated and real datasets for tailing analysis. Moreover, to show the broad utility of Tailor, we used Tailor to reanalyze published datasets and revealed novel findings worth further experimental validation. The source code and the executable binaries are freely available at https://github.com/jhhung/Tailor.

Categories: Journal Articles

Nucleotidyl transferase assisted DNA labeling with different click chemistries

Nucleic Acids Research - Tue, 09/29/2015 - 01:41

Here, we present a simple, modular and efficient strategy that allows the 3'-terminal labeling of DNA, regardless of whether it has been chemically or enzymatically synthesized or isolated from natural sources. We first incorporate a range of modified nucleotides at the 3'-terminus, using terminal deoxynucleotidyl transferase. In the second step, we convert the incorporated nucleotides, using either of four highly efficient click chemistry-type reactions, namely copper-catalyzed azide-alkyne cycloaddition, strain-promoted azide-alkyne cycloaddition, Staudinger ligation or Diels-Alder reaction with inverse electron demand. Moreover, we create internal modifications, making use of either ligation or primer extension, after the nucleotidyl transferase step, prior to the click reaction. We further study the influence of linker variants on the reactivity of azides in different click reactions. We find that different click reactions exhibit distinct substrate preferences, a fact that is often overlooked, but should be considered when labeling oligonucleotides or other biomolecules with click chemistry. Finally, our findings allowed us to extend our previously published RNA labeling strategy to the use of a different copper-free click chemistry, namely the Staudinger ligation.

Categories: Journal Articles

A novel hybrid single molecule approach reveals spontaneous DNA motion in the nucleosome

Nucleic Acids Research - Tue, 09/29/2015 - 01:41

Structural dynamics of nucleic acid and protein is an important physical basis of their functions. These motions are often very difficult to synchronize and too fast to be clearly resolved with the currently available single molecule methods. Here we demonstrate a novel hybrid single molecule approach combining stochastic data analysis with fluorescence correlation that enables investigations of sub-ms unsynchronized structural dynamics of macromolecules. Based on the method, we report the first direct evidence of spontaneous DNA motions at the nucleosome termini. The nucleosome, comprising DNA and a histone core, is the fundamental packing unit of eukaryotic genes that must be accessed during various genome transactions. Spontaneous DNA opening at the nucleosome termini has long been hypothesized to enable gene access in the nucleosome, but has yet to be directly observed. Our approach reveals that DNA termini in the nucleosome open and close repeatedly at 0.1–1 ms–1. The kinetics depends on salt concentration and DNA–histone interactions but not much on DNA sequence, suggesting that this dynamics is universal and imposes the kinetic limit to gene access. These results clearly demonstrate that our method provides an efficient and robust means to investigate unsynchronized structural changes of DNA at a sub-ms time resolution.

Categories: Journal Articles

A modular open platform for systematic functional studies under physiological conditions

Nucleic Acids Research - Tue, 09/29/2015 - 01:41

Any profound comprehension of gene function requires detailed information about the subcellular localization, molecular interactions and spatio-temporal dynamics of gene products. We developed a multifunctional integrase (MIN) tag for rapid and versatile genome engineering that serves not only as a genetic entry site for the Bxb1 integrase but also as a novel epitope tag for standardized detection and precipitation. For the systematic study of epigenetic factors, including Dnmt1, Dnmt3a, Dnmt3b, Tet1, Tet2, Tet3 and Uhrf1, we generated MIN-tagged embryonic stem cell lines and created a toolbox of prefabricated modules that can be integrated via Bxb1-mediated recombination. We used these functional modules to study protein interactions and their spatio-temporal dynamics as well as gene expression and specific mutations during cellular differentiation and in response to external stimuli. Our genome engineering strategy provides a versatile open platform for efficient generation of multiple isogenic cell lines to study gene function under physiological conditions.

Categories: Journal Articles
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