Dengue virus NS5 protein plays multiple functions in the cytoplasm of infected cells, enabling viral RNA replication and counteracting host antiviral responses. Here, we demonstrate a novel function of NS5 in the nucleus where it interferes with cellular splicing. Using global proteomic analysis of infected cells together with functional studies, we found that NS5 binds spliceosome complexes and modulates endogenous splicing as well as minigene-derived alternative splicing patterns. In particular, we show that NS5 alone, or in the context of viral infection, interacts with core components of the U5 snRNP particle, CD2BP2 and DDX23, alters the inclusion/exclusion ratio of alternative splicing events, and changes mRNA isoform abundance of known antiviral factors. Interestingly, a genome wide transcriptome analysis, using recently developed bioinformatics tools, revealed an increase of intron retention upon dengue virus infection, and viral replication was improved by silencing specific U5 components. Different mechanistic studies indicate that binding of NS5 to the spliceosome reduces the efficiency of pre-mRNA processing, independently of NS5 enzymatic activities. We propose that NS5 binding to U5 snRNP proteins hijacks the splicing machinery resulting in a less restrictive environment for viral replication.
Light signaling pathways and the circadian clock interact to help organisms synchronize physiological and developmental processes with periodic environmental cycles. The plant photoreceptors responsible for clock resetting have been characterized, but signaling components that link the photoreceptors to the clock remain to be identified. Here we describe a family of night lightinducible and clock-regulated genes (LNK) that play a key role linking light regulation of gene expression to the control of daily and seasonal rhythms in Arabidopsis thaliana. A genomewide transcriptome analysis revealed that most light-induced genes respond more strongly to light during the subjective day, which is consistent with the diurnal nature of most physiological processes in plants. However, a handful of genes, including the homologous genes LNK1 and LNK2, are more strongly induced by light in the middle of the night, when the clock is most responsive to this signal. Further analysis revealed that the morning phased LNK1 and LNK2 genes control circadian rhythms, photomorphogenic responses, and photoperiodic dependent flowering, most likely by regulating a subset of clock and flowering time genes in the afternoon. LNK1 and LNK2 themselves are directly repressed by members of the TIMING OF CAB1 EXPRESSION/PSEUDO RESPONSE REGULATOR family of core-clock genes in the afternoon and early night. Thus, LNK1 and LNK2 integrate early light signals with temporal information provided by core oscillator components to control the expression of afternoon genes, allowing plants to keep track of seasonal changes in day length.
The mechanisms by which poikilothermic organisms ensure that biological processes are robust to temperature changes are largely unknown. Temperature compensation, the ability of circadian rhythms to maintain a relatively constant period over the broad range of temperatures resulting from seasonal fluctuations in environmental conditions, is a defining property of circadian networks. Temperature affects the alternative splicing (AS) of several clock genes in fungi, plants, and flies, but the splicing factors that modulate these effects to ensure clock accuracy throughout the year remain to be identified. Here we show that GEMIN2, a spliceosomal small nuclear ribonucleoprotein assembly factor conserved from yeast to humans, modulates low temperature effects on a large subset of pre-mRNA splicing events. In particular, GEMIN2 controls the AS of several clock genes and attenuates the effects of temperature on the circadian period in Arabidopsis thaliana. We conclude that GEMIN2 is a key component of a posttranscriptional regulatory mechanism that ensures the appropriate acclimation of plants to daily and seasonal changes in temperature conditions. spliceosome assembly | alternative splicing | circadian rhythms | Arabidopsis | GEMIN2 C ircadian clocks allow organisms to coordinate physiological processes with periodic environmental changes. The core of all circadian systems, in organisms ranging from cyanobacteria to humans, is a network of multiple interlocked feedback loops that operate at the transcriptional, translational, and posttranslational levels to sustain oscillations with a period of ∼24 h, even in the absence of environmental cues. An increasing body of evidence links alternative splicing (AS) with the regulation of circadian networks across eukaryotic organisms (1-3). The core clock genes period in Drosophila, frequency in Neurospora, and BMAL2 in humans undergo AS to give rise to different mRNA isoforms (1, 2, 4). In Arabidopsis, several core clock genes, including TIMING OF CAB EXPRESSION 1 (TOC1) and CIRCA-DIAN CLOCK ASSOCIATED 1 (CCA1), also undergo extensive AS (5-7).Interestingly, many of the alternative mRNA isoforms associated with the Arabidopsis core clock genes are abundant or alter their abundance upon changes in environmental conditions, suggesting that they have important physiological roles (5-7). For example, there is strong evidence that temperature regulation of CCA1 AS is critical for the proper functioning of circadian rhythms under cold conditions (8). Temperature also regulates the AS of frequency in Neurospora and period in Drosophila (1, 2), thereby promoting the proper functioning of circadian networks under the wide range of temperatures occurring throughout the seasons. Although our knowledge of the transcription factors that regulate clock function in different organisms has increased drastically over the last two decades, the splicing factors that modulate the AS patterns of core clock genes are only starting to be characterized (1). Splicing factors that mediate the effects...
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