Youshan Yang scite author profile

Neuronal stressors such as hypoxia and firing of action potentials at very high frequencies cause intracellular Na+ to rise and ATP to be consumed faster than it can be regenerated. We report the cloning of a gene encoding a K+ channel, Slick, and demonstrate that functionally it is a hybrid between two classes of K+ channels, Na+-activated (KNa) and ATP-sensitive (KATP) K+ channels. The Slick channel is activated by intracellular Na+ and Cl- and is inhibited by intracellular ATP. Slick is widely expressed in the CNS and is detected in heart. We identify a consensus ATP binding site near the C terminus of the channel that is required for ATP and its nonhydrolyzable analogs to reduce open probability. The convergence of Na+, Cl-, and ATP sensitivity in one channel may endow Slick with the ability to integrate multiple indicators of the metabolic state of a cell and to adjust electrical activity appropriately.

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How Does the W434F Mutation Block Current in Shaker Potassium Channels?

Yang

1997

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The mutation W434F produces an apparently complete block of potassium current in Shaker channels expressed in Xenopus oocytes. Tandem tetrameric constructs containing one or two subunits with this mutation showed rapid inactivation, although the NH2-terminal inactivation domain was absent from these constructs. The inactivation showed a selective dependence on external cations and was slowed by external TEA; these properties are characteristic of C-type inactivation. Inactivation was, however, incompletely relieved by hyperpolarization, suggesting the presence of a voltage-independent component. The hybrid channels had near-normal conductance and ion selectivity. Single-channel recordings from patches containing many W434F channels showed occasional channel openings, consistent with open probabilities of 10−5 or less. We conclude that the W434F mutation produces a channel that is predominantly found in an inactivated state.

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Determination of a Comprehensive Alternative Splicing Regulatory Network and Combinatorial Regulation by Key Factors during the Epithelial-to-Mesenchymal Transition

Yang

Park

Bebee

et al. 2016

Molecular and Cellular Biology

131

165

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fThe epithelial-to-mesenchymal transition (EMT) is an essential biological process during embryonic development that is also implicated in cancer metastasis. While the transcriptional regulation of EMT has been well studied, the role of alternative splicing (AS) regulation in EMT remains relatively uncharacterized. We previously showed that the epithelial cell-type-specific proteins epithelial splicing regulatory proteins 1 (ESRP1) and ESRP2 are important for the regulation of many AS events that are altered during EMT. However, the contributions of the ESRPs and other splicing regulators to the AS regulatory network in EMT require further investigation. Here, we used a robust in vitro EMT model to comprehensively characterize splicing switches during EMT in a temporal manner. These investigations revealed that the ESRPs are the major regulators of some but not all AS events during EMT. We determined that the splicing factor RBM47 is downregulated during EMT and also regulates numerous transcripts that switch splicing during EMT. We also determined that Quaking (QKI) broadly promotes mesenchymal splicing patterns. Our study highlights the broad role of posttranscriptional regulation during the EMT and the important role of combinatorial regulation by different splicing factors to fine tune gene expression programs during these physiological and developmental transitions.A lternative splicing (AS) is a process by which a single gene transcript can be differentially spliced to yield numerous splice variants that can encode different protein isoforms and thereby greatly expand the protein coding capacity of the genome. Nearly all human genes are alternatively spliced, and cell-typespecific protein isoforms have been shown to be functionally essential for cell fate and viability (1-3). This process is under complex regulation by various cis elements in pre-mRNAs and their cognate binding partners, mainly RNA-binding proteins (RBPs). Splicing-regulatory RBPs recruited to their respective binding sites can have positive or negative effects on the splicing of different exons or splice sites. Many RBPs with largely ubiquitous expression in different tissues and cells have been shown to have broad impacts on splicing and important cell functions, such as SR and hnRNP protein families (4). However, several tissue-specific RBPs, such as NOVA, PTBP2 (nPTB), MBNL, and RBFOX proteins, have recently been described as having important roles as essential regulators of tissue-or cell-type-specific splicing (5-9). In order to further define a "splicing code" that controls broad patterns of tissue-specific splicing, as well as those that occur during developmental transitions, it is essential to characterize in greater detail how these tissue-specific regulators fine-tune AS programs combinatorially with more ubiquitously expressed splicing regulators (10).The epithelial-to-mesenchymal transition (EMT) is a process by which epithelial cells transdifferentiate into mesenchymal cells, which involves extensive changes at the cellular ...

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Single-Channel Properties of IKs Potassium Channels

1998

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Expressed in Xenopus oocytes, KvLQT1 channel subunits yield a small, rapidly activating, voltage- dependent potassium conductance. When coexpressed with the minK gene product, a slowly activating and much larger potassium current results. Using fluctuation analysis and single-channel recordings, we have studied the currents formed by human KvLQT1 subunits alone and in conjunction with human or rat minK subunits. With low external K+, the single-channel conductances of these three channel types are estimated to be 0.7, 4.5, and 6.5 pS, respectively, based on noise analysis at 20 kHz bandwidth of currents at +50 mV. Power spectra computed over the range 0.1 Hz–20 kHz show a weak frequency dependence, consistent with current interruptions occurring on a broad range of time scales. The broad spectrum causes the apparent single-channel current value to depend on the bandwidth of the recording, and is mirrored in very “flickery” single-channel events of the channels from coexpressed KvLQT1 and human minK subunits. The increase in macroscopic current due to the presence of the minK subunit is accounted for by the increased apparent single-channel conductance it confers on the expressed channels. The rat minK subunit also confers the property that the outward single-channel current is increased by external potassium ions.

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Youshan Yang

Slick (Slo2.1), a Rapidly-Gating Sodium-Activated Potassium Channel Inhibited by ATP

How Does the W434F Mutation Block Current in Shaker Potassium Channels?

Determination of a Comprehensive Alternative Splicing Regulatory Network and Combinatorial Regulation by Key Factors during the Epithelial-to-Mesenchymal Transition

Single-Channel Properties of IKs Potassium Channels

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