Saccharomyces cerevisiae Mutants Affected in Vacuole Assembly or Vacuolar H+-ATPase are Hypersensitive to Lead (Pb) Toxicity

Lead is an important environmental pollutant. The role of vacuole, in Pb detoxification, was studied using a vacuolar protein sorting mutant strain (vps16D), belonging to class C mutants. Cells disrupted in VPS16 gene, did not display a detectable vacuolar-like structure. Based on the loss of cell proliferation capacity, it was found that cells from vps16D mutant exhibited a hypersensitivity to Pb-induced toxicity, compared to wild type (WT) strain. The function of vacuolar H?-ATPase (VATPase), in Pb detoxification, was evaluated using mutants with structurally normal vacuoles but defective in subunits of catalytic (vma1D or vma2D) or membrane domain (vph1D or vma3D) of V-ATPase. All mutants tested, lacking a functional V-ATPase, displayed an increased susceptibility to Pb, comparatively to cells from WT strain. Modification of vacuolar morphology, in Pb-exposed cells, was visualized using a Vma2p-GFP strain. The treatment of yeast cells with Pb originated the fusion of the medium size vacuolar lobes into one enlarged vacuole. In conclusion, it was found that vacuole plays an important role in the detoxification of Pb in Saccharomyces cerevisiae; in addition, a functional V-ATPase was required for Pb compartmentalization.

Sarcoplasmic reticulum calcium ATPase is inhibited by organic vanadium coordination compounds: pyridine-2,6-dicarboxylatodioxovanadium(V), BMOV, and an amavadine analogue

Inorg Chem. 2008 Jul 7;47(13):5677-84. doi: 10.1021/ic702405d

Importancia del Ca2+ en la fisiolog��a esperm��tica: modulaci��n de su actividad por progesterona y prote��nas del plasma seminal. Importance of calcium in sperm physiology: its regulation by progesterone and proteins from the seminal plasma.

El objetivo general del proyecto es estudiar el efecto de la progesterona y de algunas prote��nas del plasma seminal sobre la actividad del Ca2+ en diferentes procesos fisiol��gicos que ocurren en el espermatozoide, los cuales est��n estrechamente relacionados con la capacidad fertilizante de esta c��lula. La progesterona, principal esteroide secretado por las c��lulas del cumulus oophorus, ejerce su efecto a trav��s de un receptor no-gen��mico provocando aumento en el calcio intracelular de los espermatozoides y, consecuentemente, promoviendo la capacitaci��n, la respuesta quimiot��ctica y la exocitosis acrosomal. Pese a estas observaciones, los mecanismos a trav��s de los cuales la progesterona estimula fen��menos tan diversos en el espermatozoide son a��n desconocidos. Tampoco se conoce con exactitud el papel funcional y los mecanismos de acci��n de algunas prote��nas del plasma seminal que interaccionan y se unen a los espermatozoides, con alta especificidad, durante la eyaculaci��n. Por lo tanto, resulta altamente interesante profundizar los estudios sobre las propiedades funcionales de las prote��nas caltrin (calcium transport inhibitor) y ��-microseminoprotein (MSP) del plasma seminal de mam��feros, las cuales responden a las caracter��sticas mencionadas. Los estudios hasta ahora realizados han dado cuenta de que caltrin inhibe la incorporaci��n de Ca2+ extracelular, previene la exocitosis acrosomal espont��nea y promueve la uni��n espermatozoide-zona pel��cida. Tambi��n hay datos preliminares que sugieren un efecto inhibitorio sobre la movilidad hiperactivada de los espermatozoides. Respecto a MSP, s��lo se sabe que inhibe la exocitosis acrosomal espont��nea y que su contenido, en el plasma seminal, guarda una relaci��n inversa con la fertilidad. Por todo lo expuesto, se propone estudiar los mecanismos de acci��n de la progesterona y las prote��nas caltrin y MSP sobre los procesos fisiol��gicos antes indicados. Para ello, se estudiar��n las variaciones de Ca2+ intracelular en espermatozoides individuales sometidos a diferentes tratamientos (gradientes de progesterona, capacitaci��n en presencia y ausencia de caltrin y/o MSP, etc.), usando video microscop��a de fluorescencia y an��lisis computarizado de im��genes. Tambi��n se examinar�� la influencia de estas mol��culas sobre la interacci��n de gametas y la fertilizaci��n.

Mecanismo de interacci��n, calcio dependiente, entre Calcineurina y PERK, involucrado en el Estr��s de Ret��culo Endopl��smico. Ca2+ -dependent mechanism of interaction between Calcineurin and PERK involved in Endoplasmic Reticulum Stress.

El Estr��s de Ret��culo Endopl��smico (RE) es inducido por la acumulaci��n de prote��nas sin plegar en el lumen de la organela. Esto se puede observar en diversas situaciones fisio-patol��gicas como durante una infecci��n viral o en proceso isqu��mico. Adem��s, contribuye a la base molecular de numerosas enfermedades ya sea ��ndole metab��lico (Fibrosis qu��stica o Diabetes Miellitus) o neurodegenerativas como mal de Alzheimer o Parkinson (Mutat Res, 2005, 569). Para restablecer la homeostasis en la organela se activa una se��al de transducci��n (UPR), cuya respuesta inmediata es la atenuaci��n de la s��ntesis de prote��na debido a la fosforilaci��n de subunidad alpha del factor eucari��tico de iniciaci��n de translaci��n (eIF2��) v��a PERK. Esta es una prote��na de membrana de RE que detecta estr��s. Bajo condiciones normales, PERK est�� inactiva debido a la asociaci��n de su dominio luminar con la chaperona BIP (Nat Cell Biol, 2000, 2: 326). Frente a una situaci��n de estr��s, la chaperona se disocia causando desinhibici��n. Recientemente, (Plos One 5: e11925) se observ��, bajo condiciones de estr��s, un aumento de Ca2+ citos��lico y un r��pido incremento de la expresi��n de calcineurina (CN), una fosfatasa citos��lica dependiente de calcio, heterodim��rica formada por una subunidad catal��tica (CN-A) y una regulatoria (CN-B). Adem��s, CN interacciona, sin intermediarios, con el dominio citos��lico de PERK favoreciendo su trans-autofosforilaci��n. Resultados preliminares indican que, astrocitos CNA��-/- exhibieron, en condiciones basales, un mayor n��mero de c��lulas muertas y de niveles de eIF2�� fosforilado que los astrocitos CNA��-/-. Hip��tesis: CNA��/B interacciona con PERK cuando el Ca2+ citos��lico esta incrementado luego de haberse inducido Estr��s de RE, lo cual promueve dimerizaci��n y auto-fosforilaci��n de la quinasa, acentu��ndose as�� la fosforilaci��n de eIF2�� e inhibici��n de la s��ntesis de prote��nas. Esta activaci��n citos��lica de PERK colaborar��a con la ya descrita, desinhibici��n luminal llevada cabo por BIP. Cuando el Ca2+ citos��lico retorna a los niveles basales, PERK fosforila a CN, reduciendo su afinidad de uni��n y disoci��ndose el complejo CN/PERK. Objetivo general: Definir las condiciones por las cuales CN interacciona con PERK y regula la fosforilaci��n de eIF2�� e inhibici��n de la s��ntesis de prote��na. Objetivos espec��ficos: I-Estudiar la diferencia de afinidades y dependencia de Ca2+, de las dos isoformas de CN (�� y ��) en su asociaci��n con PERK. Adem��s verificar la posible participaci��n de la subunidad B de CN en esta interacci��n. II-Determinar si la auto-fosforilaci��n de PERK es diferencialmente regulada por las dos isoformas de CN. III-Discernir la relaci��n del estado de fosforilaci��n de CN con su uni��n a PERK. IV-Determinar efectos fisiol��gicos de la interacci��n de CN-PERK durante la respuesta de Estr��s de RE. Para llevar a cabo este proyecto se realizar��n experimentos de biolog��a molecular, interacci��n prote��na-prote��na, ensayos de fosforilaci��n in vitro y un perfil de polisoma con astrocitos CNA��-/- , CNA���-/- y astrocitos controles. Se espera encontrar una mayor afinidad de uni��n a PERK de la isoforma �� de CN y en condiciones donde la concentraci��n de Ca2+ sea del orden micromolar e imite niveles del i��n durante un estr��s. Con respecto al estado de fosforilaci��n de CN, debido a los resultados preliminares, donde solo se la encontr�� fosforilada en condiciones basales, se piensa que CN podr��a interactuar con mayor afinidad con PERK cuando CN se encuentre desfosforilada. Por ��ltimo, se espera encontrar un aumento de eIF2�� fosforilado y una acentuaci��n de la atenuaci��n de la s��ntesis de prote��na como consecuencia de la mayor activaci��n de PERK por su asociaci��n con la isoforma �� de CN en astrocitos donde el Estr��s de RE se indujo por privaci��n de oxigeno y glucosa. Estos experimentos permitir��n avanzar en el estudio de una nueva funci��n citoprotectora de CN recientemente descrita por nuestro grupo de trabajo y sus implicancias en un modelo de isquemia. The accumulation of unfolded proteins into the Endoplasmic Reticulum (ER) activates a signal transduction cascade called Unfolding Protein Response (UPR), which attempts to restore homeostasis in the organelle. (PKR)-like-ER kinase (PERK) is an early stress response transmembrane protein that is generally inactive due to its association with the chaperone BIP. During ER stress, BIP is tritrated by the unfolded protein, leading PERK activation and phosphorylation of eukaryotic initiation factor-2 alpha (eIF2alpha), which attenuates protein s��ntesis. If ER damage is too great and homeostasis is not restored within a certain period of time, an apoptotic response is elicited. We recently demonstrated a cytosolic Ca2+ increase in Xenopus oocytes after induce ER stress. Moreover, calcineurin A/B, a an heterotrimeric Ca2+ dependent phosphatases (CN-A/B), associates with PERK increasing its auto-phosphorylation and significantly enhancing cell viability. Preliminary results suggest that, CN-A��-/- knockout astrocytes exhibit a significant higher eIF2�� phosphorylated level compared to CN-A��-/- astrocytes. Our working hypothesis establishes that: CN binds to PERK when cytosolic Ca2+ is initially increased by ER stress, promoting dimerization and autophosphorylation, which leads to phosphorylation of elF2�� and subsequently attenuation of protein translation. When cytosolic Ca2+ returns to resting levels, PERK phosphorylates CN, reducing its binding affinity so that the CN/PERK complex dissociates. The goal of this project is to determine the conditions by which CN binding to PERK attenuates protein translation during the ER stress response and subsequently, to determine how the interaction of CN with PERK is terminated when stress is removed. To perform this project is planed to do molecular biology experiments, pull down assays, in vitro phosphorylations and assess overall mRNA translation efficiency doing a polisome profile.

Exerc��cio e restri����o alimentar aumentam o RNAm de prote��nas do tr��nsito de Ca2+ mioc��rdico em ratos

FUNDAMENTO: Treinamento f��sico (TF) aumenta a sensibilidade dos horm��nios tireoidianos (HT) e a express��o g��nica de estruturas moleculares envolvidas no movimento intracelular de c��lcio do mioc��rdio, enquanto a restri����o alimentar (RIA) promove efeitos contr��rios ao TF. OBJETIVO: Avaliar os efeitos da associa����o TF e RIA sobre os n��veis plasm��ticos dos HT e a produ����o de mRNA dos receptores HT e estruturas moleculares do movimento de c��lcio do mioc��rdio de ratos. M��TODOS: Utilizaram-se ratos Wistar Kyoto divididos em: controle (C, n = 7), RIA (R50, n = 7), exerc��cio f��sico (EX, n = 7) e exerc��cio f��sico + RIA (EX50, n = 7). A RIA foi de 50% e o TF foi nata����o (1 hora/dia, cinco sess��es/semana, 12 semanas consecutivas). Avaliaram-se as concentra����es s��ricas de triiodotironina (T3), tiroxina (T4) e horm��nio tireotr��fico (TSH). O mRNA da bomba de c��lcio do ret��culo sarcoplasm��tico (SERCA2a), fosfolamban (PLB), trocador Na+/Ca+2 (NCX), canal lento de c��lcio (canal-L), rianodina (RYR), calsequestrina (CQS) e receptor de HT (TRα1 e TRβ1) do mioc��rdio foram avaliados por rea����o em cadeia da polimerase (PCR) em tempo real. RESULTADOS: RIA reduziu o T4, TSH e mRNA do TRα1 e aumentou a express��o da PLB, NCX e canal-L. TF aumentou a express��o do TRβ1, canal-L e NCX. A associa����o TF e RIA reduziu T4 e TSH e aumentou o mRNA do TRβ1, SERCA2a, NCX, PLB e correla����o do TRβ1 com a CQS e NCX. CONCLUS��O: Associa����o TF e RIA aumentou o mRNA das estruturas moleculares c��lcio transiente, por��m o eixo HT-receptor n��o parece participar da transcri����o g��nica dessas estruturas.

Remodelamento mioc��rdico ap��s grandes infartos converte potencia����o p��s-pausa em decaimento da for��a em ratos

FUNDAMENTO: A Contra����o P��s-Repouso (CPR) do m��sculo card��aco fornece informa����es indiretas sobre a manipula����o de c��lcio intracelular. OBJETIVO: Nosso objetivo foi estudar o comportamento da CPR e seus mecanismos subjacentes em camundongos com infarto do mioc��rdio. M��TODOS: Seis semanas ap��s a oclus��o coronariana, a contratilidade dos M��sculos Papilares (MP) obtidos a partir de camundongos submetidos �� cirurgia sham (C, n = 17), com infarto moderado (MMI, n = 10) e grande infarto (LMI, n = 14), foi avaliada ap��s intervalos de repouso de 10 a 60 segundos antes e depois da incuba����o com cloreto de l��tio (Li+) em substitui����o ao cloreto de s��dio ou rianodina (Ry). A express��o proteica de SR Ca(2+)-ATPase (SERCA2), trocador Na+/Ca2+ (NCX), fosfolambam (PLB) e fosfo-Ser (16)-PLB foi analisada por Western blotting. RESULTADOS: Os camundongos MMI apresentaram potencia����o de CPR reduzida em compara����o aos camundongos C. Em oposi����o �� potencia����o normal para camundongos C, foram observadas degrada����es de for��a p��s-repouso nos m��sculos de camundongos LMI. Al��m disso, a Ry bloqueou a degrada����o ou potencia����o de PRC observada em camundongos LMI e C; o Li+ inibiu o NCX e converteu a degrada����o em potencia����o de CPR em camundongos LMI. Embora os camundongos MMI e LMI tenham apresentado diminui����o no SERCA2 (72 �� 7% e 47 �� 9% de camundongos controle, respectivamente) e express��o prot��ica de fosfo-Ser16-PLB (75 �� 5% e 46 �� 11%, respectivamente), a superexpress��o do NCX (175 �� 20%) s�� foi observada nos m��sculos de camundongos LMI. CONCLUS��O: Nossos resultados mostraram, pela primeira vez, que a remodela����o mioc��rdica p��s-IAM em camundongos pode mudar a potencia����o regular para degrada����o p��s-repouso, afetando as prote��nas de manipula����o de Ca(2+) em mi��citos.

Chronic Stress Improves NO- and Ca2+ Flux-Dependent Vascular Function: A Pharmacological Study

Background: Stress is associated with cardiovascular diseases. Objective: This study aimed at assessing whether chronic stress induces vascular alterations, and whether these modulations are nitric oxide (NO) and Ca2+ dependent. Methods: Wistar rats, 30 days of age, were separated into 2 groups: control (C) and Stress (St). Chronic stress consisted of immobilization for 1 hour/day, 5 days/week, 15 weeks. Systolic blood pressure was assessed. Vascular studies on aortic rings were performed. Concentration-effect curves were built for noradrenaline, in the presence of L-NAME or prazosin, acetylcholine, sodium nitroprusside and KCl. In addition, Ca2+ flux was also evaluated. Results: Chronic stress induced hypertension, decreased the vascular response to KCl and to noradrenaline, and increased the vascular response to acetylcholine. L-NAME blunted the difference observed in noradrenaline curves. Furthermore, contractile response to Ca2+ was decreased in the aorta of stressed rats. Conclusion: Our data suggest that the vascular response to chronic stress is an adaptation to its deleterious effects, such as hypertension. In addition, this adaptation is NO- and Ca2+-dependent. These data help to clarify the contribution of stress to cardiovascular abnormalities. However, further studies are necessary to better elucidate the mechanisms involved in the cardiovascular dysfunction associated with stressors. (Arq Bras Cardiol. 2014; [online].ahead print, PP.0-0)

Obesity Resistance Promotes Mild Contractile Dysfunction Associated with Intracellular Ca2+ Handling

Abstract Background: Diet-induced obesity is frequently used to demonstrate cardiac dysfunction. However, some rats, like humans, are susceptible to developing an obesity phenotype, whereas others are resistant to that. Objective: To evaluate the association between obesity resistance and cardiac function, and the impact of obesity resistance on calcium handling. Methods: Thirty-day-old male Wistar rats were distributed into two groups, each with 54 animals: control (C; standard diet) and obese (four palatable high-fat diets) for 15 weeks. After the experimental protocol, rats consuming the high-fat diets were classified according to the adiposity index and subdivided into obesity-prone (OP) and obesity-resistant (OR). Nutritional profile, comorbidities, and cardiac remodeling were evaluated. Cardiac function was assessed by papillary muscle evaluation at baseline and after inotropic maneuvers. Results: The high-fat diets promoted increase in body fat and adiposity index in OP rats compared with C and OR rats. Glucose, lipid, and blood pressure profiles remained unchanged in OR rats. In addition, the total heart weight and the weight of the left and right ventricles in OR rats were lower than those in OP rats, but similar to those in C rats. Baseline cardiac muscle data were similar in all rats, but myocardial responsiveness to a post-rest contraction stimulus was compromised in OP and OR rats compared with C rats. Conclusion: Obesity resistance promoted specific changes in the contraction phase without changes in the relaxation phase. This mild abnormality may be related to intracellular Ca2+ handling.

Mitochondrial ultrastructural and atpase changes during the life cycle of Ascaris Suum

Ultrastructural morphology and ATPase specific activities of mitochondria isolated from 1-celled fertilized egg, 10-day embryo, 21-day infective larvae and adult body wall muscle of Ascaris suum and rat liver were determined and compared. Although cristae of both muscle and egg mitochondria contained numerous elementary particles with head pieces of conventional diameter (85 A), each muscle mitochondrion contained relatively few, short cristae with a diminished frequency of elementary particles and associated ATPase activity. These morphological relationships are related to the previous conclusion that the transition from an aerobic to an essentially anaerobic metabolism is intimately associated with the mitochondrion and is a normal and mandatory feature of development.

The fourth extracellular loop of the alpha subunit of Na,K-ATPase. Functional evidence for close proximity with the second extracellular loop.

Na,K-ATPase is the main active transport system that maintains the large gradients of Na(+) and K(+) across the plasma membrane of animal cells. The crystal structure of a K(+)-occluding conformation of this protein has been recently published, but the movements of its different domains allowing for the cation pumping mechanism are not yet known. The structure of many more conformations is known for the related calcium ATPase SERCA, but the reliability of homology modeling is poor for several domains with low sequence identity, in particular the extracellular loops. To better define the structure of the large fourth extracellular loop between the seventh and eighth transmembrane segments of the alpha subunit, we have studied the formation of a disulfide bond between pairs of cysteine residues introduced by site-directed mutagenesis in the second and the fourth extracellular loop. We found a specific pair of cysteine positions (Y308C and D884C) for which extracellular treatment with an oxidizing agent inhibited the Na,K pump function, which could be rapidly restored by a reducing agent. The formation of the disulfide bond occurred preferentially under the E2-P conformation of Na,K-ATPase, in the absence of extracellular cations. Using recently published crystal structure and a distance constraint reproducing the existence of disulfide bond, we performed an extensive conformational space search using simulated annealing and showed that the Tyr(308) and Asp(884) residues can be in close proximity, and simultaneously, the SYGQ motif of the fourth extracellular loop, known to interact with the extracellular domain of the beta subunit, can be exposed to the exterior of the protein and can easily interact with the beta subunit.

The potassium impermeable apical membrane of insect epithelia: a target for development of safe pesticides

Columnar cell apical membranes (CCAM) in series with goblet cell apical membranes (GCAM) form an electroosmotic barrier separating the midgut lumen from epithelial cell cytoplasm. A unique K+ ATPase in GCAM generates three gradients across this barrier. A greater than 180 mV electrical gradient (lumen positive) drives amino acid uptake through voltage-dependent K+ symports. A greater than 1000-fold [H+] gradient (lumen alkaline) and a greater than 10-fold [K+] gradient (lumen concentrated) are adaptations to the high tannin and high K+ content, respectively, in dietary plant material. Agents which act on the apical membrane and disrupt the PD, H+, or K+ gradients are potential insecticides. Insect sensory epithelia and mammalian stria vascularis maintain similar PD and K+ gradients but would not be exposed to ingested anti-apical membrane insecticides. Following the demonstration by Sacchi et al. that Bacillus thuringiensis delta-endotoxin (Bt) induces specifically a K+ conductance increase in CCAM vesicles, we find that the K+ channel blocking agent, Ba2+, completely reverses Bt inhibition of the K+-carried short circuit current in the isolated midgut of Manduca sexta. Progress in characterizing the apical membrane includes finding that fluorosulfonylbenzoyladenosine binds specifically to certain GCAM polypeptides and that CCAM vesicles can be mass produced by Ca2+ or Mg2+ precipitation from Manduca sexta midgut.

T-type Ca2+ channels, SK2 channels and SERCAs gate sleep-related oscillations in thalamic dendrites.

T-type Ca2+ channels (T channels) underlie rhythmic burst discharges during neuronal oscillations that are typical during sleep. However, the Ca2+-dependent effectors that are selectively regulated by T currents remain unknown. We found that, in dendrites of nucleus reticularis thalami (nRt), intracellular Ca2+ concentration increases were dominated by Ca2+ influx through T channels and shaped rhythmic bursting via competition between Ca2+-dependent small-conductance (SK)-type K+ channels and Ca2+ uptake pumps. Oscillatory bursting was initiated via selective activation of dendritically located SK2 channels, whereas Ca2+ sequestration by sarco/endoplasmic reticulum Ca2+-ATPases (SERCAs) and cumulative T channel inactivation dampened oscillations. Sk2-/- (also known as Kcnn2) mice lacked cellular oscillations, showed a greater than threefold reduction in low-frequency rhythms in the electroencephalogram of non-rapid-eye-movement sleep and had disrupted sleep. Thus, the interplay of T channels, SK2 channels and SERCAs in nRt dendrites comprises a specialized Ca2+ signaling triad to regulate oscillatory dynamics related to sleep.

Separate neuronal and glial Na+,K+-ATPase isoforms regulate glucose utilization in response to membrane depolarization and elevated extracellular potassium.

The role of cell type-specific Na+,K+-ATPase isozymes in function-related glucose metabolism was studied using differentiated rat brain cell aggregate cultures. In mixed neuron-glia cultures, glucose utilization, determined by measuring the rate of radiolabeled 2-deoxyglucose accumulation, was markedly stimulated by the voltage-dependent sodium channel agonist veratridine (0.75 micromol/L), as well as by glutamate (100 micromol/L) and the ionotropic glutamate receptor agonist N-methyl-D-aspartate (NMDA) (10 micromol/L). Significant stimulation also was elicited by elevated extracellular potassium (12 mmol/L KCl), which was even more pronounced at 30 mmol/L KCl. In neuron-enriched cultures, a similar stimulation of glucose utilization was obtained with veratridine, specific ionotropic glutamate receptor agonists, and 30 mmol/L but not 12 mmol/L KCl. The effects of veratridine, glutamate, and NMDA were blocked by specific antagonists (tetrodotoxin, CNQX, or MK801, respectively). Low concentrations of ouabain (10(-6) mol/L) prevented stimulation by the depolarizing agents but reduced only partially the response to 12 mmol/L KCl. Together with previous data showing cell type-specific expression of Na+,K+-ATPase subunit isoforms in these cultures, the current results support the view that distinct isoforms of Na+,K+-ATPase regulate glucose utilization in neurons in response to membrane depolarization, and in glial cells in response to elevated extracellular potassium.

The fourth transmembrane segment of the Na,K-ATPase alpha subunit: a systematic mutagenesis study.

The Na,K-ATPase is a major ion-motive ATPase of the P-type family responsible for many aspects of cellular homeostasis. To determine the structure of the pathway for cations across the transmembrane portion of the Na,K-ATPase, we mutated 24 residues of the fourth transmembrane segment into cysteine and studied their function and accessibility by exposure to the sulfhydryl reagent 2-aminoethyl-methanethiosulfonate. Accessibility was also examined after treatment with palytoxin, which transforms the Na,K-pump into a cation channel. Of the 24 tested cysteine mutants, seven had no or a much reduced transport function. In particular cysteine mutants of the highly conserved "PEG" motif had a strongly reduced activity. However, most of the non-functional mutants could still be transformed by palytoxin as well as all of the functional mutants. Accessibility, determined as a 2-aminoethyl-methanethiosulfonate-induced reduction of the transport activity or as inhibition of the membrane conductance after palytoxin treatment, was observed for the following positions: Phe(323), Ile(322), Gly(326), Ala(330), Pro(333), Glu(334), and Gly(335). In accordance with a structural model of the Na,K-ATPase obtained by homology modeling with the two published structures of sarcoplasmic and endoplasmic reticulum calcium ATPase (Protein Data Bank codes 1EUL and 1IWO), the results suggest the presence of a cation pathway along the side of the fourth transmembrane segment that faces the space between transmembrane segments 5 and 6. The phenylalanine residue in position 323 has a critical position at the outer mouth of the cation pathway. The residues thought to form the cation binding site II ((333)PEGL) are also part of the accessible wall of the cation pathway opened by palytoxin through the Na,K-pump.

Functional effects of Na+,K+-ATPase gene mutations linked to familial hemiplegic migraine.

Familial hemiplegic migraine type 2, an autosomal dominant form of migraine with aura, has been associated with four distinct mutations in the alpha2-subunit of the Na+,K+-ATPase. We have introduced these mutations in the alpha2-subunit of the human Na+,K+-ATPase and the corresponding mutations in the Bufo marinus alpha1-subunit and studied these mutants by expression in Xenopus oocyte. Metabolic labeling studies showed that the mutants were synthesized and associated with the beta-subunit, except for the alpha2HW887R mutant, which was poorly synthesized, and the alpha1BW890R, which was partially retained in the endoplasmic reticulum. [3H]ouabain binding showed the presence of the alpha2HR689Q and alpha2HM731T at the membrane, whereas the alpha2HL764P and alpha2HW887R could not be detected. Functional studies with the mutants of the B. marinus Na+,K+-ATPase showed a reduced or abolished electrogenic activity and a low K+ affinity for the alpha1BW890R mutant. Through different mechanisms, all these mutations result in a strong decrease of the functional expression of the Na+,K+-pump. The decreased activity in alpha2 isoform of the Na+,K+-pump expressed in astrocytes seems an essential component of hemiplegic migraine pathogenesis and may be responsible for the cortical spreading depression, which is one of the first events in migraine attacks.