论文信息 - Decreased expression of Kv4.2 and novel Kv4.3 K+ channel subunit mRNAs in ventricles of renovascular hypertensive rats.

Decreased expression of Kv4.2 and novel Kv4.3 K+ channel subunit mRNAs in ventricles of renovascular hypertensive rats.

Hypertension-induced cardiac hypertrophy is associated with alterations in ventricular action potentials. To understand molecular mechanisms underlying this electrical abnormality, expression of cardiac voltage-gated K+ channel subunit genes was examined in ventricles of renovascular hypertensive rats. While generating a rat Kv4.3 probe, we discovered a previously unreported 19-amino acid insertion in the C-terminal intracellular region of the channel subunit. RNase protection assays indicated that this novel isoform is predominant in rat lung and heart. Effects of renovascular hypertension were then determined by using renal artery clipping models: two-kidney, one clip (2K-1C) rats, a model of high-renin hypertension with a normal plasma volume, and one-kidney, one clip (1K-1C) rats, a model of normal renin with a raised plasma volume. Expression of Kv4.2 and Kv4.3 mRNAs was diminished by > 50% in ventricles of 2K-1C rats; however, no changes in the expression of Kv1.2, Kv1.4, Kv1.5, Kv2.1, or KvLQT1 mRNAs were detected. Similar downregulation of Kv4.2 and Kv4.3 mRNAs was detected in 1K-1C rats. Chronic administration of captopril, an angiotensin-converting enzyme inhibitor, blocked the development of hypertension and the suppression of Kv4 subfamily channel mRNA expression in 2K-1C rats. Furthermore, captopril administration to sham-operated rats significantly increased Kv4.2 mRNA. These results indicate that renovascular hypertension causes specific reductions in Kv4 subfamily channel mRNA expression and that this effect is likely to be mediated primarily by an increase in cardiac afterload.

[1] G. Gintant,et al. Tissue and species distribution of mRNA for the IKr-like K+ channel, erg. , 1997, Circulation research.

[2] K. Takimoto,et al. Dexamethasone and Stress Upregulate Kv1.5 K+ Channel Gene Expression in Rat Ventricular Myocytes , 1996, Neuropharmacology.

[3] M. Sanguinetti,et al. Coassembly of KVLQT1 and minK (IsK) proteins to form cardiac IKS potassium channel , 1996, Nature.

[4] Jacques Barhanin,et al. KvLQT1 and IsK (minK) proteins associate to form the IKS cardiac potassium current , 1996, Nature.

[5] N. El-Sherif,et al. Differential expression of voltage-gated K+ channel genes in left ventricular remodeled myocardium after experimental myocardial infarction. , 1996, Circulation research.

[6] D. Mckinnon,et al. Role of the Kv4.3 K+ channel in ventricular muscle. A molecular correlate for the transient outward current. , 1996, Circulation research.

[7] D Qin,et al. Cellular and ionic basis of arrhythmias in postinfarction remodeled ventricular myocardium. , 1996, Circulation research.

[8] L. Dell’Italia,et al. Cardiac hypertrophy and failure in hypertension. , 1996, Current opinion in nephrology and hypertension.

[9] G. Landes,et al. Positional cloning of a novel potassium channel gene: KVLQT1 mutations cause cardiac arrhythmias , 1996, Nature Genetics.

[10] Depressed transient outward current in single hypertrophied cardiomyocytes isolated from the right ventricle of ferret heart. , 1995, Cardiovascular research.

[11] J. Nerbonne,et al. Differential expression of voltage-gated K+ channel subunits in adult rat heart. Relation to functional K+ channels? , 1995, Circulation Research.

[12] H. Shear,et al. Characterization of a voltage-gated K+ channel beta subunit expressed in human heart. , 1995, Proceedings of the National Academy of Sciences of the United States of America.

[13] H. Strauss,et al. A Novel β Subunit Increases Rate of Inactivation of Specific Voltage-gated Potassium Channel α Subunits (*) , 1995, The Journal of Biological Chemistry.

[14] B. Wible,et al. Molecular cloning and functional expression of a novel potassium channel β‐subunit from human atrium , 1995 .

[15] P. Boyden,et al. Ion channel function in disease. , 1995, Cardiovascular research.

[16] K. Takimoto,et al. Glucocorticoid induction of Kv1.5 K+ channel gene expression in ventricle of rat heart. , 1994, Circulation research.

[17] B. Rudy,et al. Identification of molecular components of A-type channels activating at subthreshold potentials. , 1994, Journal of neurophysiology.

[18] A Mugelli,et al. Ionic basis of action potential prolongation of hypertrophied cardiac myocytes isolated from hypertensive rats of different ages. , 1994, Cardiovascular research.

[19] R. Myerburg,et al. Diminished transient outward currents in rat hypertrophied ventricular myocytes. , 1994, Circulation research.

[20] D. Mckinnon,et al. Quantitative analysis of potassium channel mRNA expression in atrial and ventricular muscle of rats. , 1994, Circulation research.

[21] M. Gammage,et al. Hypertension and the heart. , 1994, British medical bulletin.

[22] H. Matsubara,et al. The transcription of a mammalian voltage-gated potassium channel is regulated by cAMP in a cell-specific manner. , 1993, The Journal of biological chemistry.

[24] J. D. Da Ponte,et al. Heterogeneity of the early outward current in ventricular cells isolated from normal and hypertrophied rat hearts. , 1993, The Journal of physiology.

[25] J. Trimmer,et al. Dexamethasone rapidly induces Kv1.5 K+ channel gene transcription and expression in clonal pituitary cells , 1993, Neuron.

[26] K. Takimoto,et al. Organization and characterization of the rat class 3 aldehyde dehydrogenase gene. , 1993, The Journal of biological chemistry.

[27] A J Levi,et al. The electrophysiological characteristics of hypertrophied ventricular myocytes from the spontaneously hypertensive rat , 1993, Journal of hypertension.

[28] K. Takimoto,et al. Glucocorticoid induced up-regulation of a pituitary K+ channel mRNA in vitro and in vivo. , 1993, Receptors & channels.

[29] Mark Ellisman,et al. Region-specific expression of a K+ channel gene in brain. , 1992, Proceedings of the National Academy of Sciences of the United States of America.

[30] B. Rudy,et al. Cloning of ShIII (Shaw-like) cDNAs encoding a novel high-voltage-activating, TEA-sensitive, type-A K+ channel , 1992, Proceedings of the Royal Society of London. Series B: Biological Sciences.

[31] W. Kannel. Left ventricular hypertrophy as a risk factor: the Framingham experience , 1991, Journal of hypertension. Supplement : official journal of the International Society of Hypertension.

[32] T. J. Baldwin,et al. Characterization of a mammalian cDNA for an inactivating voltage-sensitive K+ channel , 1991, Neuron.

[33] E. Levitan,et al. Alternative splicing contributes to K+ channel diversity in the mammalian central nervous system. , 1991, Proceedings of the National Academy of Sciences of the United States of America.

[34] X. Xu,et al. Decreased transient outward K+ current in ventricular myocytes from acromegalic rats. , 1991, The American journal of physiology.

[35] S. Roberds,et al. Cloning and tissue-specific expression of five voltage-gated potassium channel cDNAs expressed in rat heart. , 1991, Proceedings of the National Academy of Sciences of the United States of America.

[36] L. Kaczmarek,et al. Cloning and expression of cDNA and genomic clones encoding three delayed rectifier potassium channels in rat brain , 1990, Neuron.

[37] B. Sakmann,et al. Molecular basis of functional diversity of voltage‐gated potassium channels in mammalian brain. , 1989, The EMBO journal.

[38] A. VanDongen,et al. A novel potassium channel with delayed rectifier properties isolated from rat brain by expression cloning , 1989, Nature.

[39] E. Keung,et al. Calcium current is increased in isolated adult myocytes from hypertrophied rat myocardium. , 1989, Circulation research.

[40] S. Houser,et al. Calcium currents in normal and hypertrophied isolated feline ventricular myocytes. , 1988, The American journal of physiology.

[41] P. Chomczyński,et al. Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. , 1987, Analytical biochemistry.