Gill-specific transcriptional regulation of Na+/K+-ATPase {alpha}-subunit in the euryhaline shore crab Pachygrapsus marmoratus: sequence variants and promoter structure

doi:10.1242/jeb.004309

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First published online June 11, 2007
Journal of Experimental Biology 210, 2070-2081 (2007)
Published by The Company of Biologists 2007
doi: 10.1242/jeb.004309

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Gill-specific transcriptional regulation of Na⁺/K⁺-ATPase ${alpha}$ -subunit in the euryhaline shore crab Pachygrapsus marmoratus: sequence variants and promoter structure

Nishad Jayasundara¹^,*, David W. Towle¹^,, Dirk Weihrauch² and Céline Spanings-Pierrot³

¹ Center for Marine Functional Genomics, Mount Desert Island Biological Laboratory, Salsbury Cove, ME 04672, USA
² Division of Animal Physiology, University of Osnabrück, D-49076 Osnabrück, Germany
³ Université Montpellier II, Adaptation Ecophysiologique et Ontogenese, UMR 5119 CP092, Pl. E. Bataillon, 34095 Montpellier cédex 5, France

Author for correspondence (e-mail: dtowle{at}mdibl.org)

Accepted 27 March 2007

Summary

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Summary
Introduction
Materials and methods
Results
Discussion
References

The sodium pump (Na⁺/K⁺-ATPase) has been implicated in osmoregulatoryion transport in many aquatic animals. In the euryhaline hyper–hypoosmoregulatingshore crab Pachygrapsus marmoratus, induction of Na⁺/K⁺-ATPase ${alpha}$ -subunit mRNA varies between gills in response to osmotic stress.Following transfer of crabs from normal seawater (36 ${per thousand}$ salinity)to diluted seawater (10 ${per thousand}$ ), a condition in which gills exhibitnet ion uptake, ${alpha}$ -subunit mRNA expression is upregulated in alltested gills, albeit with differing time courses. By contrast,following transfer from seawater to hypertonic (45 ${per thousand}$ ) seawater,a condition in which the animal is excreting ions, ${alpha}$ -subunitmRNA is induced primarily in gill no. 7 (nine in total), suggestingthat this gill may be associated specifically with ion excretionin P. marmoratus.

Full-length sequencing of ${alpha}$ -subunit cDNA revealed the existenceof two isoforms differing only in the inclusion of an 81-nucleotidesegment within the N-terminal open reading frame of the long(D) form in comparison to the short (C) form. The 81-nucleotidesegment encodes a 14-3-3 protein binding site that may facilitatemovement of the ${alpha}$ -subunit protein between intracellular compartmentsand the plasma membrane. mRNA expression of the two forms followedsimilar patterns upon salinity transfer. Genomic DNA sequencing ofthe putative promoter region of the ${alpha}$ -subunit gene demonstrateda spectrum of predicted transcription factor binding sites thatare likely associated with the complex expression pattern observedamong gills following osmotic stress.

Key words: crab gill, osmoregulation, real-time quantitative PCR, salinity, sequence variants, sodium pump, ${alpha}$ -subunit

Introduction

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Summary
Introduction
Materials and methods
Results
Discussion
References

The cellular mechanisms by which euryhaline animals adjust tochanges in environmental salinity are beginning to be exploredat the level of gene expression. A number of candidate ion transporterand transport-related genes have been identified in osmoregulatorytissues of euryhaline species and their cDNAs have been sequenced,including Na⁺/K⁺-ATPase ${alpha}$ -subunit (Cutler et al., 1995; Towleet al., 2001), Na⁺/H⁺ exchangers (Towle et al., 1997; Choe etal., 2005), Na⁺/K⁺/2Cl^– cotransporter (Pelis et al., 2001; Luquetet al., 2005; Scott et al., 2005), cystic fibrosis transmembraneregulator (Singer et al., 1998), V-type H⁺-ATPase (Weihrauchet al., 2001; Luquet et al., 2005), aquaporins (Cutler and Cramb, 2002;Lignot et al., 2002) and carbonic anhydrase (Henry et al., 2003).

In this study, we examined the expression of mRNA encoding thecatalytic ${alpha}$ -subunit of Na⁺/K⁺-ATPase, a transmembrane proteinlocalized in the basolateral membrane of most animal epithelialcells, where it uses energy derived from ATP hydrolysis to movethree Na⁺ ions from the cytosol to the cell exterior in exchangefor two K⁺ ions, thus establishing an electrochemical gradientacross the cell membrane that drives secondary active transportprocesses (Skou and Esmann, 1992; Lopina, 2000; Kaplan, 2002).In hyperosmoregulatory epithelia, basolateral Na⁺/K⁺-ATPase isthought to drive apical uptake of Na⁺ from a dilute medium into theepithelial cells and across the basolateral membrane into theblood (Lucu and Towle, 2003; Evans et al., 2005). In aquaticanimals capable of hypoosmoregulation, such as some marine teleosts, basolateralNa⁺/K⁺-ATPase is believed to indirectly energize excretion ofions via a Na⁺/K⁺/2Cl^– cotransporter or other secondarytransport mechanisms (Perry, 1997; Evans et al., 2005).

It has been known for many years that the enzymatic activityof Na⁺/K⁺-ATPase in gills of euryhaline species is responsiveto environmental salinity, generally increasing in situationsthat demand greater osmoregulatory ion transport. For example,in the killifish Fundulus heteroclitus, Na⁺/K⁺-ATPase activity ingills is substantially higher in hypoosmoregulating seawater-acclimated animalsthan in hyperosmoregulating freshwater-acclimated animals (Epsteinet al., 1967), and enzymatic activity in both conditions ishigher than in animals acclimated to brackish water where littlenet salt transport is required (Towle et al., 1977). Among euryhalinecrustaceans, gill Na⁺/K⁺-ATPase activity also responds to salinity,the highest activity being generally observed in reduced salinitiesin which the animals hyperosmoregulate their hemolymph (e.g. Towleet al., 1976; Neufeld et al., 1980; Siebers et al., 1982; Harrisand Bayliss, 1988; Lucu and Flik, 1999). In particular, theposterior gills of euryhaline brachyurans exhibit significantlyhigher Na⁺/K⁺-ATPase activity than anterior gills, in agreementwith the observed abundance of basolateral membrane infoldingsin epithelial cells of posterior gills (Copeland and Fitzjarrell, 1968;Goodman and Cavey, 1990).

It has been unclear whether the adaptive changes in Na⁺/K⁺-ATPaseactivity were the result of enzymatic activation or synthesisand/or recruitment of new membrane-bound protein. Increasesin the abundance of mRNA encoding the Na⁺/K⁺-ATPase ${alpha}$ -subunithave been noted in gills of brown trout following seawater transfer (Madsenet al., 1995), in European sea bass following transfer from15 ${per thousand}$ salinity to either freshwater or seawater (Jensen et al., 1998),and in the killifish transferred from 10 ${per thousand}$ salinity to freshwater,whereas a transient increase was observed after transfer to seawaterin this species (Scott et al., 2004). Na⁺/K⁺-ATPase ${alpha}$ -subunitmRNA levels have been shown to increase in posterior gills ofthe South American crab Chasmagnathus granulatus following transferfrom isosmotic conditions (30 ${per thousand}$ salinity) to either dilute (2 ${per thousand}$ )or concentrated (45 ${per thousand}$ ) seawater (Luquet et al., 2005) and in posteriorgills of the blue crab Callinectes sapidus after transfer from32 ${per thousand}$ to 10 ${per thousand}$ (Lovett et al., 2006).

However, little attention has been given to ascertaining differencesin gene expression in individual gills, although measurementsof transport function and Na⁺/K⁺-ATPase activity following salinity challengein euryhaline crabs, suggest important functional differences betweengills (Siebers et al., 1982; Wanson et al., 1984; Welcomme andDevos, 1988; Martinez et al., 1998). In addition, there is littleinformation regarding possible transcription factors and theirbinding sites that may be associated with transcriptional regulationof the Na⁺/K⁺-ATPase in crustaceans.

The marble shore crab Pachygrapsus marmoratus is strongly euryhaline,transporting environmental NaCl across the gill from low salinitiesand thus maintaining a hyperosmotic hemolymph in dilute seawater. At33 ${per thousand}$ salinity, the hemolymph of P. marmoratus is essentially isosmoticwith the medium. At 10 ${per thousand}$ salinity, however, the hemolymph of P.marmoratus is regulated at approximately 550 mOsmol kg^–1above the osmolality of the medium (Pierrot et al., 1995). Unlike manybrachyuran crabs, this species is also capable of excretingNaCl into high salinity environments, thereby maintaining ahypoosmotic hemolymph in concentrated seawater. At 45 ${per thousand}$ salinity,for example, the osmotic concentration of the hemolymph is regulatedat approximately 250 mOsmol kg^–1 below that of the medium (Pierrotet al., 1995).

The capacity for ion transport in isolated gills of this speciesis enhanced by treatment with neurohormonal extracts that maymediate the organismal response to salinity change, in partby stimulating changes in Na⁺/K⁺-ATPase activity (Eckhardt etal., 1995; Spanings-Pierrot et al., 2000). Like other brachyurancrabs, the gills are morphologically and functionally distinct:the anterior gills are thought to be specialized for gas exchangeand the posterior gills for ion transport (Pierrot, 1996). Therefore, P.marmoratus is an excellent model in which to study the dynamicsof environmentally influenced transporter gene expression inosmoregulatory tissues that show functional differentiation.

The objective of the present work was to focus on one of themain ion transporters, the Na⁺/K⁺-ATPase, by amplifying and sequencingNa⁺/K⁺-ATPase ${alpha}$ -subunit cDNA from gills of P. marmoratus andby measuring salinity-related ${alpha}$ -subunit mRNA expression in individualgills from crabs subjected to salinity stress using real-timequantitative PCR, a technique for profiling gene expression quantitatively(Bustin et al., 2005). Sequencing of upstream promoter regionsin the ${alpha}$ -subunit gene revealed potential transcription factorbinding sites that may function in transcriptional regulation.

Materials and methods

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Summary
Introduction
Materials and methods
Results
Discussion
References

Animals and tissue sampling
Specimens of the marble shore crab Pachygrapsus marmoratus Fabricius1787 were caught on rocky areas of the Mediterranean coast ofFrance near Montpellier and transported to UniversitéMontpellier II where they were kept at 20±1°C inindividual compartments containing recirculating natural seawaterat 36 ${per thousand}$ salinity. A 12 h:12 h light:dark photoperiod was maintained.They were fed three times a week with pieces of mussels. Priorto experimentation, food was withdrawn for 48 h. Crabs in intermoltstage C (Drach and Tchernigovtzeff, 1967) were transferred toeither 10 ${per thousand}$ salinity (seawater diluted with dechlorinated freshwater) or 45 ${per thousand}$ salinity (seawater supplemented with syntheticsea salts, Reef Crystals, Instant Ocean, Sarrebourg, France).At intervals of 2, 4, 6, 24 and 48 h, crabs were sacrificedfollowing anesthesia on ice and individual gills were dissectedand immediately placed into RNAlater (Ambion, Cambridge, UK),yielding separate samples of the largest gills in the branchialchamber, i.e. the last two pairs of anterior gills (numbers5 and 6) and the three pairs of posterior gills (7, 8 and 9).Gills 1–4 were of insufficient size to work with individuallyand were not used in this study. Dissected gills were transportedin RNAlater to the Mount Desert Island Biological Laboratorywhere molecular analyses were carried out.

RNA and DNA extraction, cDNA synthesis and sequencing
Total RNA was extracted from numbered gills pooled from threeto four animals under RNAse-free conditions (Chomczynski andSacchi, 1987) with materials supplied by Promega (RNAgents TotalRNA Isolation System, Madison, WI, USA). Because high qualityRNA and normalization to total RNA are essential to producingbiologically relevant and reliable data using real-time PCR(Bustin et al., 2005), each RNA extract was analyzed for qualityand quantity by microfluidic electrophoresis with an Agilent2100 Bioanalyzer (Waldbronn, Germany). Two micrograms of eachsample of total RNA were reverse transcribed to single-strandedcDNA with SuperScript II reverse transcriptase (Invitrogen, Carlsbad,CA, USA) using oligo(dT) as primer.

A partial cDNA sequence encoding the ${alpha}$ -subunit of P. marmoratusNa⁺/K⁺-ATPase was initially amplified by PCR from gill cDNAemploying degenerate primers NAK10F and NAK16R that were basedon conserved sequences from other species (Towle et al., 2001) (Table 1).Following an initial hot start at 91°C for 5 min, amplificationwas performed for 30 cycles of 94°C for 1 min, 45°Cfor 1 min and 72°C for 2 min, followed by 1 cycle of 72°Cfor 5 min and storage at 4°C. Following gel purification (MinEluteGel Extraction, Qiagen, Valencia, CA, USA) and dideoxynucleotide sequencing(ABI Prism 3100, Foster City, CA, USA), a 707-nucleotide sequence wasobtained, confirmed by BLAST analysis (Altschul et al., 1997)as a partial Na⁺/K⁺-ATPase ${alpha}$ -subunit cDNA sequence. Primers specificto this sequence, designed using Primer Premier software, wereemployed in the completion of P. marmoratus ${alpha}$ -subunit cDNA sequencingusing 3'-RACE (Invitrogen) and 5'-RACE (Clontech, Palo Alto,CA, USA) techniques. To differentiate problematic amplificationsin the 5' region of the cDNA, PCR products were subcloned usingTA cloning (Invitrogen) and inserts in individual plasmid preparationswere then sequenced. A multiple alignment and phylogenetic treeof ${alpha}$ -subunit nucleotide sequences were produced using the MegAligncomponent of DNASTAR software and open reading frames were predictedusing DNASIS software.

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Table 1. Composition of oligonucleotide primers employed in initial amplification, genomic DNA sequencing, and quantitative PCR analysis of Na⁺/K⁺-ATPase ${alpha}$ -subunit isoforms and arginine kinase cDNA in gills of Pachygrapsus marmoratus

Genomic DNA was isolated from P. marmoratus gills and testisusing a DNeasy Tissue Kit (Qiagen). The segment of genomic DNAencoding the upstream promoter region, the probable transcriptionstart site, and the 5' region of the mRNA transcript of theNa⁺/K⁺-ATPase ${alpha}$ -subunit were amplified and sequenced using aGenomeWalker Kit (Clontech) (Fors et al., 1990) with reverseprimers (PMNAK238R and PMNAK583R; Table 1) based initially onthe ${alpha}$ -subunit cDNA sequence with subsequent primers designedas necessary. Putative transcription factor binding sites werepredicted using MatInspector (Cartharius et al., 2005), transcriptionelement search software (TESS) (Schug and Overton, 1997), P-Match(Chekmenev et al., 2005) and TFSearch (Akiyama, 1995). Becausesome predictions could represent false positives, we includedin our analysis only putative binding sites predicted by atleast three of these programs.

Quantification of gene expression
Analysis of Na⁺/K⁺-ATPase ${alpha}$ -subunit mRNA expression was accomplishedby real-time quantitative PCR (QPCR) using SYBR green bindingwith the Brilliant QPCR Master Mix and MX4000 instrumentation (Stratagene,Cedar Creek, TX, USA). Initial experiments used primers thatwere designed to quantify the total expression of ${alpha}$ -subunit mRNA(NAKPMF1 and NAKPMR1, Table 1). Primers employed to differentiatebetween the two ${alpha}$ -subunit isoforms were PMNAKUSF, which targeteda portion of the 81-nucleotide segment present in isoform D,and PMNAKSPF, which bridged the flanking sequences around this 81-nucleotidesequence, missing in isoform C. Both of these forward primers wereused with reverse primer PMNAK238R (Table 1). The thermal profile forreal-time PCR consisted of an activation step at 95°C for15 min and 40 cycles of denaturing at 94°C for 40 s, annealingat 55°C for 40 s and elongation at 72°C for 1 min. Afterthe last amplification cycle, the temperature was increasedto 95°C for 1 min and then decreased to 55°C to run82 cycles, increasing by 0.5°C per cycle, to obtain meltingcurves, which confirmed the absence of non-specific PCR productsand primer dimers.

mRNA expression levels were normalized to total RNA contentby using triplicate 1 µl aliquots of each 20 µlcDNA reaction mixture that was produced with 2 µg totalRNA. cDNA in each QPCR incubation was thus derived from 0.1µg total RNA. One reference gill preparation shown toexhibit high expression levels (gill 6 at 48 h exposure to 10 ${per thousand}$ salinity) served as the basis for a standard dilution series,demonstrating a linear relationship between threshold cycle(C_t) and log₁₀ of template availability, and was used as thebasis for calculating relative abundance values in the remainingsamples. Expression of Na⁺/K⁺-ATPase ${alpha}$ -subunit mRNA was comparedto that of a putative housekeeping gene, arginine kinase (Kotlyaret al., 2000), using primers specific to P. marmoratus argininekinase cDNA (Table 1).

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Fig. 1. Multiple alignment and phenogram of initial 707-nucleotide amplification product of Na⁺/K⁺-ATPase ${alpha}$ -subunit from Pachygrapsus marmoratus (accession no. AF375957) with corresponding partial cDNA sequences from four other arthropods: blue crab Callinectes sapidus (acc. no. AF327439), American lobster Homarus americanus (acc. no. AY140650), mosquito Anopheles gambiae (acc. no. XM_563283), and honey bee Apis mellifera (acc. no. XM_392363). The alignment (A) and phenogram (B) were both generated using the Hein algorithm (Hein, 1990

) in the MegAlign component of DNASTAR software and configured with GeneDoc (Nicholas and Nicholas, 1997

). The blue background indicates 100% agreement between all five sequences, green 80%, and yellow 60%. Bootstrap values at each node of the phenogram=100.

Statistics
Statistical analyses of time course data were performed by two-wayANOVA with Bonferroni post-hoc test of differences from zerotime (data from crabs in 36 ${per thousand}$ seawater). Statistical significancewas accepted if P<0.05.

Results

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Summary
Introduction
Materials and methods
Results
Discussion
References

The initial amplification product of 707 nucleotides revealeda close match with Na⁺/K⁺-ATPase ${alpha}$ -subunit cDNA sequences from otherarthropod species upon BLAST analysis and multiple alignment (Fig. 1).The partial nucleotide sequence obtained from Pachygrapsus marmoratusmost closely resembled the Na⁺/K⁺-ATPase ${alpha}$ -subunit cDNA sequenceof another euryhaline, brachyuran crab Callinectes sapidus (accessionno. AF327439) (Towle et al., 2001) and was somewhat less similarto the corresponding sequence of a more stenohaline decapodcrustacean Homarus americanus (acc. no. AY140650). The two selectedinsect ${alpha}$ -subunit sequences were grouped separately by the alignmentprotocol.

We completed the sequencing of the ${alpha}$ -subunit cDNA using 3'- and 5'-RACEtechniques and primers based on the sequence of the initial amplificationproduct. An incomplete sequence of 1554 nucleotides was initiallysubmitted to NCBI (Accession No. AF375957). Finishing out the 3'end proved to be straightforward, requiring only the designof additional primers for primer walking. However, completionof the 5' end was more problematic, producing two amplificationproducts in situations where one was expected. We became convincedthat in fact there are two ${alpha}$ -subunit cDNA sequences in P. marmoratusgills, differing only in the inclusion of 81 nucleotides inthe so-called `D' form that are absent in the `C' form. Theadditional 81 nucleotides in the longer D form reside closeto the probable translation start site. The two mRNA sequencesare predicted to lead to the production of two different ${alpha}$ -subunitproteins varying in size by 27 amino acids (Fig. 2).

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Fig. 2. Complete nucleotide and predicted amino acid sequence of the D form (accession no. DQ173924) of Na⁺/K⁺-ATPase ${alpha}$ -subunit cDNA amplified from gills of Pachygrapsus marmoratus. The C form (acc. no. DQ173925) lacks the 81-nucleotide segment and 27-amino-acid segment indicated in blue. A consensus 14-3-3 binding site RTDSYR (Aitken, 2002

), indicated by a rectangle, is found near the N terminus of the D form but not the C form. In-frame stop codons are indicated in red. Ten transmembrane domains predicted by transmembrane hidden Markov modeling (TMHMM) (Sonnhammer et al., 1998

) are underlined. Prosite (release 20.3) analysis identified the amino acid sequence DKTGTLT at position 390-396 (bold typeface) as a characteristic P-type ATPase motif including the aspartate that becomes phosphorylated during the transport cycle (Kaplan, 2002

). A cAMP- and cGMP-dependent protein kinase phosphorylation site (RRNS) is predicted at position 954-957 (bold typeface). Brackets enclose the 707-nucleotide section initially amplified and aligned in Fig. 1 with corresponding segments from other species.

Analysis of the two ${alpha}$ -subunit protein sequences indicate thatboth contain the same ten transmembrane domains predicted bytransmembrane hidden Markov modeling (TMHMM) (Sonnhammer et al.,1998

), consistent with topologies based on experimental and computationalanalyses (Kaplan, 2002

) (Fig. 2). Prosite analysis (release20.3) revealed the amino acid sequence DKTGTLT at position 390-396containing the trademark P-type ATPase motif including the aspartatethat becomes phosphorylated during the reaction cycle (Kaplan,2002

). A single cAMP- and cGMP-dependent protein kinase phosphorylationsite was also identified at position 954-957. An inspectionof the two amino acid sequences using the eukaryote linear motif(ELM) resource for functional sites in proteins (Puntervollet al., 2003

) revealed a most interesting distinction betweenthe C and D forms of the ${alpha}$ -subunit. In the extended D form, thesequence of 27 additional amino acids contains the motif RTDSYR,identified by ELM as a putative binding site for the regulatoryprotein 14-3-3 (Mackintosh, 2004

) (Fig. 2).

A BLAST search (Altschul et al., 1997) of the `non-redundant'and `other EST' databases of GenBank revealed cDNAs or expressedsequence tags from other crustacean species corresponding toboth C and D forms of the ${alpha}$ -subunit (Fig. 3). The amino acid sequenceencoded by an expressed sequence tag from the shrimp Litopenaeus vannamei(O'Leary et al., 2006) matched the C form of P. marmoratus,whereas a second EST independently obtained from Fenneropenaeuschinensis (Wang et al., 2006) matched the D form. In the onlycrustacean genome currently being sequenced, that of Daphniapulex, five ${alpha}$ -subunit encoding genes are predicted by the semi-HMM-basednucleic acid parser (SNAP) (Korf, 2004; Colbourne et al., 2005). However,none of these appear to encode an N terminus similar to thatfound in the P. marmoratus D form. By contrast, ${alpha}$ -subunit N termini containinga putative binding site for 14-3-3 are found in many other species, includingthe honeybee Apis mellifera (acc. no. XP_623072), sea urchinStrongylocentrotus purpuratus (acc. no. XP_795226), and zebrafishDanio rerio (acc. no. AAG27058) (Rajarao et al., 2001).

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Fig. 3. Multiple alignment of N-terminal amino acids of eight crustacean Na⁺/K⁺-ATPase ${alpha}$ -subunits illustrating two groups, one composed of sequences containing a 14-3-3 protein binding site (RTDSY) close to the N terminus and the other group truncated and lacking this binding site. Accession numbers are given in parentheses: Artemia franciscana Alpha1 (X56650) (Macías et al., 1991

), Artemia franciscana Alpha2 (Y07513) (Baxter-Lowe et al., 1989

), Pachygrapsus marmoratus C form (DQ173925) (present study), Litopenaeus vannamei EST (CK572083) (O'Leary et al., 2006

), P. marmoratus D form (DQ173924) (present study), Fenneropenaeus chinensis EST (BM303114) (Wang et al., 2006

), Callinectes sapidus (AF327439) (Towle et al., 2001

), Homarus americanus (AY140650) (Parrie and D.W.T., unpublished). The alignment was produced with Multalin version 5.4.1 (Corpet, 1988

) and processed with GeneDoc (Nicholas and Nicholas, 1997

). Blue background indicates 100% amino acid agreement between the eight sequences, green indicates 75–99%, yellow 50–74%.

Analysis of ${alpha}$ -subunit mRNA expression by quantitative PCR firstused primers NAKPMF1 and NAKPMR1 (Table 1) that amplified Cand D forms simultaneously. Such analysis showed a complex responseto salinity change that was gill specific and also salinityspecific. Following transfer from 36 to 10 ${per thousand}$ salinity, ${alpha}$ -subunitmRNA levels in all of the tested gills increased during the experimentalperiod, with gill 7 responding within 2 h and other gills showing adelayed response (Fig. 4A). By 24 h, all gills exhibited significantlyenhanced expression of ${alpha}$ -subunit mRNA (P<0.001). The basicpattern was repeatable in a completely independent set of gillpreparations made the following year (Fig. 4B) and demonstrateda gill-specific time course of transcript changes followingshort-term exposure to dilute salinity.

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Fig. 4. Quantitative PCR analysis of Na⁺/K⁺-ATPase ${alpha}$ -subunit mRNA abundance in individual gill preparations from Pachygrapsus marmoratus following transfer for various time periods (2–48 h) from 36 ${per thousand}$ seawater to 10 ${per thousand}$ (A,B) or to 45 ${per thousand}$ (C,D). Values are means ± s.d. (N=3 or 4 measurements at each time point using gills pooled from three or four animals) of data obtained with primers NAKPMF1 and NAKPMR1 designed to detect both isoforms simultaneously (Table 1). Two independent experiments from 2002 (A,C) and 2003 (B,D) are presented. Relative expression levels are indicated in relation to a standard reference (one sample of gill 6 at 48 h after transfer to 10 ${per thousand}$ ). Significant differences from zero time values (crabs in 36 ${per thousand}$ seawater) are indicated: *P<0.001; P<0.01.

When crabs were transferred from 36 to 45 ${per thousand}$ , a condition in whichthe animals hypoosmoregulate their hemolymph, we observed that ${alpha}$ -subunit expression remained low in all of the gills exceptfor gill 7, which showed a marked increase in ${alpha}$ -subunit mRNAwithin 6 h after the transfer, an increase that was maintainedthrough the 48-hour experimental period (Fig. 4C). This surprising resultwas confirmed in a subsequent independent experiment in thefollowing year (Fig. 4D). Our data indicate that ${alpha}$ -subunit genetranscription in gill 7 is particularly responsive to hypersalineconditions.

In many invertebrates, arginine kinase is an important componentin energy metabolism, catalyzing the phosphorylation of ADPat the expense of phosphoarginine, and it is strongly expressedin crustacean gills (Kotlyar et al., 2000). In P. marmoratus,arginine kinase mRNA levels were influenced by environmentalsalinity, but in a minor fashion compared with ${alpha}$ -subunit (Fig. 5).Transfer of crabs from 36 to 10 ${per thousand}$ salinity elicited minor butstatistically significant changes in arginine kinase mRNA levelsby 48 h after the transfer, but the pattern and extent of inductiondid not resemble that of the Na⁺/K⁺-ATPase ${alpha}$ -subunit, suggestingthat the substantial changes in ${alpha}$ -subunit mRNA expression werein specific response to the salinity challenge. Transfer ofcrabs from 36 to 45 ${per thousand}$ similarly lead to some statistically significantchanges in arginine kinase mRNA but there was no consistentpattern, even within gills, and the changes were quite smallrelative to the changes observed in ${alpha}$ -subunit expression. Interestingly,in comparison to other gills, gill 7 consistently showed thehighest level of arginine kinase mRNA, perhaps contributingto the apparently robust response of that gill to salinity stress.

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Fig. 5. Quantitative PCR analysis of arginine kinase mRNA abundance in individual gills of Pachygrapsus marmoratus transferred from 36 ${per thousand}$ to 10 ${per thousand}$ (A) or to 45 ${per thousand}$ (B) seawater for time periods indicated above the figure. Mean ± s.d. (N=3 or 4 measurements at each time point using gills pooled from three or four animals). Relative expression levels are indicated in relation to a standard reference (one sample of gill 6 at 48 h after transfer to 10 ${per thousand}$ ). Significant differences from zero time values (36 ${per thousand}$ seawater) are indicated: *P<0.001; P<0.01; P<0.05.

When we examined the differential expression of the two ${alpha}$ -subunit isoformswith respect to salinity and time course, we found more apparent variabilityamong the samples than when we analyzed total ${alpha}$ -subunit expression.Transfer of crabs from 36 to 10 ${per thousand}$ resulted in a generalized increasein transcripts encoding both isoforms, consistent with our observationsof total expression. All tested gills showed a trend toward increasedtranscript levels with longer exposure to dilute salinity, witha generally greater expression of the short isoform, C (Fig. 6A,B).However, in crabs transferred from 36 to 45 ${per thousand}$ , high expressionlevels of isoforms C and D were observed primarily in gill 7(Fig. 6C,D), in agreement with experiments measuring expressionof both isoforms simultaneously (Fig. 4C,D).

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Fig. 6. Quantitative PCR analysis of mRNA encoding C and D forms of Na⁺/K⁺-ATPase ${alpha}$ -subunit in individual gills of Pachygrapsus marmoratus transferred from 36 ${per thousand}$ seawater to 10 ${per thousand}$ (A,B) or to 45 ${per thousand}$ (C,D) seawater. Values are mean ± s.d. (N=3 measurements at each time point using gills pooled from three or four animals). Relative expression levels are indicated in relation to a standard reference (one sample of gill 6 at 48 h after transfer to 10 ${per thousand}$ ). Significant differences from zero time values (animals in 36 ${per thousand}$ seawater) are indicated: *P<0.001; P<0.01; ${ddagger}$ P<0.05.

Sequencing genomic DNA upstream of the transcription start siteof the ${alpha}$ -subunit gene using genome walking (Fors et al., 1990

)revealed a 462-nucleotide sequence adjoining the first exonthat contained four putative binding sites for the transcriptionfactor SP1, two each for ATF/CREB, AP1, and HSF, and one forMYOD (Fig. 7). Predicted CAAT and TATA box-like regions werealso identified. Sequencing genomic DNA downstream of the transcriptionstart site confirmed the existence of the short C isoform atthe genomic level, but repeated attempts to demonstrate thegenomic equivalent of the longer D isoform were unsuccessful.Amplifications of genomic DNA using primers that targeted potentialgenomic regions upstream and downstream of the predicted 81-nucleotideD-isoform inclusion consistently produced only a C-isoform amplicon.Primers targeted specifically to the 81-nucleotide inclusionitself failed to produce any product when genomic DNA was employedas template.

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Fig. 7. Genomic DNA sequence of Pachygrapsus marmoratus Na⁺/K⁺-ATPase ${alpha}$ -subunit promoter region including the transcription start site (arrow) and 462 additional upstream nucleotides determined by genome walking. CAAT and TATA box regions are shaded, and predicted binding sites for transcription factors are indicated by labeled rectangles.

	Discussion

TOP Summary Introduction Materials and methods Results Discussion References

In this study, we demonstrated the occurrence of two Na⁺/K⁺-ATPase ${alpha}$ -subunit-encoding transcripts in gills from the hyper–hypoosmoregulatingcrab Pachygrapsus marmoratus, differing only in the inclusionof an 81-nucleotide sequence near the translation start sitein the D form. Differential exon splicing in the sea urchinHemicentrotus pulcherrimus is known to produce Na⁺/K⁺-ATPase ${alpha}$ -subunit transcript variants differing only in the 5' leaderregion (Yamazaki et al., 1997

). We anticipated that the ${alpha}$ -subunitcDNA variants found in P. marmoratus were, similarly, the resultof differential exon splicing, since the only difference betweenthe two variants that we have clearly identified lies in the5' region of the sequence. We thus expected to find the D isoformin the genome, with the C isoform arising by alternative splicing.However, exhaustive analysis of genomic DNA by PCR with many combinationsof primers and amplification conditions demonstrated the existenceof only the C isoform at the genomic level. This surprisingfinding suggested to us that the 81-nucleotide addition characteristicof the D isoform might have arisen by trans-splicing, a processby which nascent pre-mRNA receives a ribonucleotide segmentencoded by genomic DNA not associated with the gene in question (Maniatisand Tasic, 2002

). However, the presence in several non-crustaceanspecies of genomic sequences encoding similar N termini ledus to conclude that the lack of success in amplifying the Dform from genomic DNA of P. marmoratus was more likely the resultof a failure to discover the proper PCR amplification conditionsrather than its actual absence.

The discovery of a predicted 14-3-3 protein binding site nearthe N-terminus of the ${alpha}$ -subunit D form of P. marmoratus and other speciessuggests that the Na⁺/K⁺-ATPase may be responsive to this regulatoryprotein in vivo. The 14-3-3 protein family binds to phosphoserineor phosphothreonine on target proteins and regulates their translocationbetween cytoplasmic or endoplasmic reticulum sites and the plasmamembrane (Dougherty and Morrison, 2004; Mackintosh, 2004). Inthe case of mammalian Na⁺/K⁺-ATPase, 14-3-3 was shown to be essentialfor the dopamine-induced endocytosis of ${alpha}$ -subunit protein in opossumkidney, apparently by binding directly to the N terminus ofthe protein (Efendiev et al., 2005). In gills of euryhalinecrabs, such a mechanism may be important in the short-term minute-by-minuteregulation of Na⁺/K⁺-ATPase function at the plasma membrane.

Longer term (hours to days) regulation of Na⁺/K⁺-ATPase functionin gills would depend, at least in part, on the availabilityof ${alpha}$ -subunit mRNA and protein. We observed significant changesin ${alpha}$ -subunit mRNA abundance following transfer from seawaterto either dilute or concentrated media, the former eliciting hyperosmoregulationof the hemolymph and the latter hypoosmoregulation. Moreover,gills responded differently both in terms of the time courseand the degree of response, indicating a gill-specific patternof transcriptional regulation. All gills examined respondedto diluted seawater, albeit with different time courses (posteriorgills generally responding more rapidly), but only gill 7 respondedto concentrated seawater. This finding by itself suggests thatall gills that we examined may participate in ion uptake from dilutemedia but only gill 7 may participate in ion excretion into concentratedmedia. The specificity of the response to a concentrated medium indicatesdistinct osmoregulatory roles among the gills, and that the increasedNa⁺/K⁺-ATPase mRNA expression is not simply part of a cellularosmoregulatory mechanism, since the cells of all of the gillswere exposed to the same salinity stress but only gill 7 responded transcriptionallyto concentrated seawater.

Such specificity of gill function in euryhaline crustaceanshas been suggested previously by studies of transport physiologyand enzyme activity. In the green shore crab Carcinus maenas,for example, individual gills show different levels of Na⁺/K⁺-ATPasespecific activity, the posterior gills generally being higherthan the anterior gills but nearly all responding to salinitychange (Siebers et al., 1982). In the mangrove crab Ucides cordatus,gill 5 (7 in total) is more permeable to sodium than gill 6;flux ratio analysis showed that gill 5 is associated with activeion uptake from dilute seawater whereas gill 6 is associatedwith active ion extrusion into concentrated seawater (Martinezet al., 1998). Our gene expression results for P. marmoratussupport the conclusion that specificity of function does indeedreside in individual gills and that gill 7 (of 9) responds toconcentrated seawater in a fashion that suggests it may be specificallyinvolved in active ion extrusion, thus facilitating hypoosmoregulationof the hemolymph.

A related study with the South American varunid crab Chasmagnathus granulatusin which Na⁺/K⁺-ATPase ${alpha}$ -subunit expression was assessed in pooledposterior (6–8) and anterior (3–5) gills showedmassive induction of transcript abundance, mainly in posteriorgills, within 24 h following transfer of crabs from 30 to 2 ${per thousand}$ salinityand by 96 h following transfer from 30 to 45 ${per thousand}$ (Luquet et al.,2005). In the portunid crab Callinectes sapidus, statisticallysignificant increases in ${alpha}$ -subunit transcript abundance appearedin a posterior gill (7) by 96 h following transfer from 32 to10 ${per thousand}$ salinity (Lovett et al., 2006), a delayed response comparedwith P. marmoratus.

The apparent complexity of transcriptional regulation of ${alpha}$ -subunit mRNAlevels in P. marmoratus suggests a corresponding complexityof promoter structure. Indeed, we show here that the promoterregion of the ${alpha}$ -subunit gene of P. marmoratus contains at leastfive different transcription factor binding sites. (Becausewe were successful in identifying only the C isoform of the ${alpha}$ -subunit at the genomic level, our description of the promoterregion refers only to that isoform.) The predicted promoterregion contains CAAT and TATA-like boxes plus a high G+C content(67%), indications that it is indeed intimately involved in transcriptionalregulation of the ${alpha}$ -subunit gene. Unlike the Na⁺/K⁺-ATPase ${alpha}$ 1-subunitgene of the branchiopod crustacean Artemia franciscana (Garcia-Sáezet al., 1997), the promoter region in P. marmoratus is contiguous withthe predicted transcription start site and thus the first exon.

Within the P. marmoratus ${alpha}$ -subunit promoter are four predictedbinding sites for stimulating protein 1 (Sp1), a common zinc-finger-liketranscription factor that interacts with CpG islands during transcriptionalregulation. Two binding sites are predicted for activator protein1 (AP1). These transcription factor binding sites are also foundin the promoter region of the ${alpha}$ 1-subunit gene of A. franciscana (Garcia-Sáezet al., 1997) as well as in mammalian ${alpha}$ -subunit genes (Keryanovand Gardner, 2002). At positions –36 and –222, bindingsites for activating transcription factor/cyclic-AMP responseelement binding protein (ATF/CREB) are predicted for the P.marmoratus ${alpha}$ -subunit gene. Proteins of the ATF/CREB family areknown to regulate gene expression during cellular responsesto environmental stress (Wilkinson et al., 1996; Fawcett etal., 1999) and binding sites for them have been reported previouslyin ${alpha}$ -subunit promoter regions of several vertebrate species (Suzuki-Yagawaet al., 1992; Yu et al., 1996). In combination with other transcriptionfactor binding sites predicted for the P. marmoratus ${alpha}$ -subunitgene (Fig. 7), it is apparent that the transcriptional regulationof this gene may offer a number of alternative choices, allowingfor the complexity of mRNA response that we observed in gillswhen crabs were transferred from seawater to dilute or concentrated environments.

Acknowledgments

This study was supported by the National Science Foundation(IBN-0340622 and IOB-0543860) to D.W.T. and New InvestigatorAwards from the Mount Desert Island Biological Laboratory toC.S.-P. The authors wish to thank Ms E. Grousset and Mr F. Aujoulatfor technical help at Université Montpellier II and MsC. Smith for efficient DNA sequencing at MDIBL.

Footnotes

^* Present address: Hopkins Marine Station, Stanford University,Pacific Grove, CA 93950, USA

References

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Summary
Introduction
Materials and methods
Results
Discussion
References

Aitken, A. (2002). Functional specificity in 14-3-3 isoform interactions through dimer formation and phosphorylation. Chromosome location of mammalian isoforms and variants. Plant Mol. Biol. 50,993 -1010.[CrossRef][Medline]

Akiyama, Y. (1995). TFSEARCH: searching transcription factor binding sites. http://www.cbrc.jp/research/db/TFSEARCH.html.

Altschul, S. F., Madden, T. L., Schaffer, A. A., Zhang, J., Zhang, Z., Miller, W. and Lipman, D. J. (1997). Gapped BLAST and PSI-BLAST: a new generation of protein database search programs. Nucleic Acids Res. 25,3389 -3402.[Abstract/Free Full Text]

Baxter-Lowe, L. A., Guo, J. Z., Bergstrom, E. E. and Hokin, L. E. (1989). Molecular cloning of the Na,K-ATPase ${alpha}$ -subunit in developing brine shrimp and sequence comparison with higher organisms. FEBS Lett. 257,181 -187.[CrossRef][Medline]

Bustin, S. A., Benes, V., Nolan, T. and Pfaffl, M. W. (2005). Quantitative real-time RT-PCR – a perspective. J. Mol. Endocrinol. 34,597 -601.[Abstract/Free Full Text]

Cartharius, K., Frech, K., Grote, K., Klocke, B., Haltmeier, M., Klingenhoff, A., Frisch, M., Bayerlein, M. and Werner, T. (2005). MatInspector and beyond: promoter analysis based on transcription factor binding sites. Bioinformatics 21,2933 -2942.[Abstract/Free Full Text]

Chekmenev, D. S., Haid, C. and Kel, A. E. (2005). P-Match: transcription factor binding site search by combining patterns and weight matrices. Nucleic Acids Res. 33,W432 -W437.[Abstract/Free Full Text]

Choe, K. P., Kato, A., Hirose, S., Plata, C., Sindic, A., Romero, M. F., Claiborne, J. B. and Evans, D. H. (2005). NHE3 in an ancestral vertebrate: primary sequence, distribution, localization, and function in gills. Am. J. Physiol. 289,R1520 -R1534.

Chomczynski, P. and Sacchi, N. (1987). Single-step method of RNA isolation by acid guanidinium thiocyanate-phenol-chloroform extraction. Anal. Biochem. 162,156 -159.[Medline]

Colbourne, J. K., Singan, V. R. and Gilbert, D. G. (2005). wFleaBase: the Daphnia genome database. BMC Bioinformatics 6,45 .[CrossRef][Medline]

Copeland, D. E. and Fitzjarrell, A. T. (1968). The salt absorbing cells in the gills of the blue crab (Callinectes sapidus Rathbun) with notes on modified mitochondria. Z. Zellforsch. Mikrosk. Anat. 92,1 -22.[CrossRef][Medline]

Corpet, F. (1988). Multiple sequence alignment with hierarchical clustering. Nucleic Acids Res. 16,10881 -10890.[Abstract/Free Full Text]

Cutler, C. P. and Cramb, G. (2002). Branchial expression of an aquaporin 3 (AQP-3) homologue is downregulated in the European eel Anguilla anguilla following seawater acclimation. J. Exp. Biol. 205,2643 -2651.[Abstract/Free Full Text]

Cutler, C. P., Sanders, I. L., Hazon, N. and Cramb, G. (1995). Primary sequence, tissue specificity and expression of the Na⁺,K⁺-ATPase alpha 1 subunit in the European eel (Anguilla anguilla). Comp. Biochem. Physiol. 111B,567 -573.[CrossRef][Medline]

Dougherty, M. K. and Morrison, D. K. (2004). Unlocking the code of 14-3-3. J. Cell Sci. 117,1875 -1884.[Abstract/Free Full Text]

Drach, P. and Tchernigovtzeff, C. (1967). Sur la méthode de détermination des stades d'intermue et son application générale aux Crustacés. Vie Milieu A 18,595 -609.

Eckhardt, E., Pierrot, C., Thuet, P., Van Herp, F., Charmantier-Daures, M., Trilles, J. P. and Charmantier, G. (1995). Stimulation of osmoregulating processes in the perfused gill of the crab Pachygrapsus marmoratus (Crustacea, Decapoda) by a sinus gland peptide. Gen. Comp. Endocrinol. 99,169 -177.[CrossRef][Medline]

Efendiev, R., Chen, Z., Krmar, R. T., Uhles, S., Katz, A. I., Pedemonte, C. H. and Bertorello, A. M. (2005). The 14-3-3 protein translates the Na⁺,K⁺-ATPase ${alpha}$ ₁-subunit phosphorylation signal into binding and activation of phosphoinositide 3-kinase during endocytosis. J. Biol. Chem. 280,16272 -16277.[Abstract/Free Full Text]

Epstein, F. H., Katz, A. I. and Pickford, G. E. (1967). Sodium- and potassium-activated adenosine triphosphatase of gills: role in adaptation of teleosts to salt water. Science 156,1245 -1247.[Abstract/Free Full Text]

Evans, D. H., Piermarini, P. M. and Choe, K. P. (2005). The multifunctional fish gill: dominant site of gas exchange, osmoregulation, acid–base regulation, and excretion of nitrogenous waste. Physiol. Rev. 85, 97-177.[Abstract/Free Full Text]

Fawcett, T. W., Martindale, J. L., Guyton, K. Z., Hai, T. and Holbrook, N. J. (1999). Complexes containing activating transcription factor (ATF)/cAMP-responsive-element-binding protein (CREB) interact with the CCAAT/enhancer-binding protein (C/EBP)-ATF composite site to regulate Gadd153 expression during the stress response. Biochem. J. 339,135 -141.[CrossRef][Medline]

Fors, L., Saavedra, R. A. and Hood, L. (1990). Cloning of the shark Po promoter using a genomic walking technique based on the polymerase chain reaction. Nucleic Acids Res. 18,2793 -2799.[Abstract/Free Full Text]

Garcia-Sáez, A., Perona, R. and Sastre, L. (1997). Polymorphism and structure of the gene coding for the ${alpha}$ 1 subunit of the Artemia franciscana Na/K-ATPase. Biochem. J. 321,509 -518.[Medline]

Goodman, S. H. and Cavey, M. J. (1990). Organization of a phyllobranchiate gill from the green shore crab Carcinus maenas (Crustacea, Decapoda). Cell Tissue Res. 260,495 -505.[CrossRef]

Harris, R. R. and Bayliss, D. (1988). Gill (Na⁺+K⁺)-ATPases in decapod crustaceans: distribution and characteristics in relation to Na⁺ regulation. Comp. Biochem. Physiol. 90A,303 -308.

Hein, J. J. (1990). Unified approach to alignment and phylogenies. Meth. Enzymol. 183,626 -645.[Medline]

Henry, R. P., Gehnrich, S., Weihrauch, D. and Towle, D. W. (2003). Salinity-mediated carbonic anhydrase induction in the gills of the euryhaline green crab, Carcinus maenas. Comp. Biochem. Physiol. 136A,243 -258.

Jensen, M. K., Madsen, S. S. and Kristiansen, K. (1998). Osmoregulation and salinity effects on the expression and activity of Na⁺,K⁺-ATPase in the gills of European sea bass, Dicentrarchus labrax (L.). J. Exp. Zool. 282,290 -300.[CrossRef][Medline]

Kaplan, J. H. (2002). Biochemistry of Na,K-ATPase. Annu. Rev. Biochem. 71,511 -535.[CrossRef][Medline]

Keryanov, S. and Gardner, K. L. (2002). Physical mapping and characterization of the human Na,K-ATPase isoform, ATP1A4. Gene 292,151 -166.[CrossRef][Medline]

Korf, I. (2004). Gene finding in novel genomes. BMC Bioinformatics 5,59 .[CrossRef][Medline]

Kotlyar, S., Weihrauch, D., Paulsen, R. S. and Towle, D. W. (2000). Expression of arginine kinase enzymatic activity and mRNA in gills of the euryhaline crabs Carcinus maenas and Callinectes sapidus. J. Exp. Biol. 203,2395 -2404.[Abstract]

Lignot, J. H., Cutler, C. P., Hazon, N. and Cramb, G. (2002). Water transport and aquaporins in the European eel (Anguilla anguilla). Symp. Soc. Exp. Biol. 2002,49 -59.

Lopina, O. D. (2000). Na⁺,K⁺-ATPase: structure, mechanism, and regulation. Membr. Cell Biol. 13,721 -744.[Medline]

Lovett, D. L., Verzi, M. P., Burgents, J. E., Tanner, C. A., Glomski, K., Lee, J. J. and Towle, D. W. (2006). Expression profiles of Na⁺,K⁺-ATPase during acute and chronic hypo-osmotic stress in the blue crab Callinectes sapidus. Biol. Bull. 211,58 -65.[Abstract/Free Full Text]

Lucu, C. and Flik, G. (1999). Na⁺-K⁺-ATPase and Na⁺/Ca²⁺ exchange activities in gills of hyperregulating Carcinus maenas.Am. J. Physiol. 276,R490 -R499.[Medline]

Lucu, C. and Towle, D. W. (2003). Na⁺+K⁺-ATPase in gills of aquatic crustacea. Comp. Biochem. Physiol. 135A,195 -214.

Luquet, C. M., Weihrauch, D., Senek, M. and Towle, D. W. (2005). Induction of branchial ion transporter mRNA expression during acclimation to salinity change in the euryhaline crab Chasmagnathus granulatus J. Exp. Biol. 208,3627 -3636.[Abstract/Free Full Text]

Macías, M.-T., Palmero, I. and Sastre, L. (1991). Cloning of a cDNA encoding an Artemia franciscana Na/K ATPase ${alpha}$ -subunit. Gene 105,197 -204.[CrossRef][Medline]

Mackintosh, C. (2004). Dynamic interactions between 14-3-3 proteins and phosphoproteins regulate diverse cellular processes. Biochem. J. 381,329 -342.[CrossRef][Medline]

Madsen, S. S., Jensen, M. K., Nohr, J. and Kristiansen, K. (1995). Expression of Na⁺-K⁺-ATPase in the brown trout, Salmo trutta: In vivo modulation by hormones and seawater. Am. J. Physiol. 269,R1339 -R1345.[Medline]

Maniatis, T. and Tasic, B. (2002). Alternative pre-mRNA splicing and proteome expansion in metazoans. Nature 418,236 -243.[CrossRef][Medline]

Martinez, C. B., Harris, R. R. and Santos, M. C. (1998). Transepithelial potential differences and sodium fluxes in isolated perfused gills of the mangrove crab (Ucides cordatus). Comp. Biochem. Physiol. 120A,227 -236.

Neufeld, G. J., Holliday, C. W. and Pritchard, J. B. (1980). Salinity adaption of gill Na,K-ATPase in the blue crab, Callinectes sapidus. J. Exp. Zool. 211,215 -224.[CrossRef]

Nicholas, K. B. and Nicholas, H. B., Jr (1997). GeneDoc: a tool for editing and annotating multiple sequence alignments. http://www.nrbsc.org/gfx/genedoc/index.html.

O'Leary, N. A., Trent, H. F., III, Robalino, J., Peck, M. E. T., McKillen, D. J. and Gross, P. S. (2006). Analysis of multiple tissue-specific cDNA libraries from the Pacific whiteleg shrimp, Litopenaeus vannamei. Integr. Comp. Biol. 46,931 -939.[Abstract/Free Full Text]

Pelis, R. M., Zydlewski, J. and McCormick, S. D. (2001). Gill Na⁺-K⁺-2Cl^– cotransporter abundance and location in Atlantic salmon: effects of seawater and smolting. Am. J. Physiol. 280,R1844 -R1852.

Perry, S. F. (1997). The chloride cell: structure and function in the gills of freshwater fishes. Annu. Rev. Physiol. 59,325 -347.[CrossRef][Medline]

Pierrot, C. (1996). Osmoregulation in the euryhaline crab, Pachygrapsus marmoratus: gill physiology and neuroendocrine control. Bull. Soc. Zool. Fr. Evol. Zool. 121,295 -304.

Pierrot, C., Péqueux, A. and Thuet, P. (1995). Perfusion of gills isolated from the hyper-hyporegulating crab Pachygrapsus marmoratus (Crustacea, Decapoda): adaptation of a method. Arch. Physiol. Biochem. 103,401 -409.[Medline]

Puntervoll, P., Linding, R., Gemund, C., Chabanis-Davidson, S., Mattingsdal, M., Cameron, S., Martin, D. M., Ausiello, G., Brannetti, B., Costantini, A. et al. (2003). ELM server: a new resource for investigating short functional sites in modular eukaryotic proteins. Nucleic Acids Res. 31,3625 -3630.[Abstract/Free Full Text]

Rajarao, S. J., Canfield, V. A., Mohideen, M. A., Yan, Y. L., Postlethwait, J. H., Cheng, K. C. and Levenson, R. (2001). The repertoire of Na,K-ATPase ${alpha}$ and ß subunit genes expressed in the zebrafish, Danio rerio. Genome Res. 11,1211 -1220.[Abstract/Free Full Text]

Schug, J. and Overton, G. C. (1997). TESS: transcription element search software on the WWW.http://www.cbil.upenn.edu/tess.

Scott, G. R., Richards, J. G., Forbush, B., Isenring, P. and Schulte, P. M. (2004). Changes in gene expression in gills of the euryhaline killifish Fundulus heteroclitus after abrupt salinity transfer. Am. J. Physiol. 287,C300 -C309.[CrossRef]

Scott, G. R., Claiborne, J. B., Edwards, S. L., Schulte, P. M. and Wood, C. M. (2005). Gene expression after freshwater transfer in gills and opercular epithelia of killifish: insight into divergent mechanisms of ion transport. J. Exp. Biol. 208,2719 -2729.[Abstract/Free Full Text]

Siebers, D., Leweck, K., Markus, H. and Winkler, A. (1982). Sodium regulation in the shore crab Carcinus maenas as related to ambient salinity. Mar. Biol. 69, 37-43.[CrossRef]

Singer, T. D., Tucker, S. J., Marshall, W. S. and Higgins, C. F. (1998). A divergent CFTR homologue: highly regulated salt transport in the euryhaline teleost F. heteroclitus. Am. J. Physiol. 274,C715 -C723.[Medline]

Skou, J. C. and Esmann, M. (1992). The Na,K-ATPase. J. Bioenerg. Biomembr. 24,249 -261.[Medline]

Sonnhammer, E. L. L., von Heijne, G. and Krogh, A. (1998). A hidden Markov model for predicting transmembrane helices in protein sequences. In Proceedings of the Sixth International Conference on Intelligent Systems for Molecular Biology (ed. J. Glasgow, T. Littlejohn, F. Major, R. Lathrop, D. Sankoff and C. Sensen), pp. 175-182. Menlo Park: AAAI Press.

Spanings-Pierrot, C., Soyez, D., Van Herp, F., Gompel, M., Skaret, G., Grousset, E. and Charmantier, G. (2000). Involvement of crustacean hyperglycemic hormone in the control of gill ion transport in the crab Pachygrapsus marmoratus. Gen. Comp. Endocrinol. 119,340 -350.[CrossRef][Medline]

Suzuki-Yagawa, Y., Kawakami, K. and Nagano, K. (1992). Housekeeping Na,K-ATPase ${alpha}$ 1 subunit gene promoter is composed of multiple cis elements to which common and cell type-specific factors bind. Mol. Cell. Biol. 12,4046 -4055.[Abstract/Free Full Text]

Towle, D. W., Palmer, G. E. and Harris, J. L., III (1976). Role of gill Na⁺+K⁺-dependent ATPase in acclimation of blue crabs (Callinectes sapidus) to low salinity. J. Exp. Zool. 196,315 -322.[CrossRef]

Towle, D. W., Gilman, M. E. and Hempel, J. D. (1977). Rapid modulation of gill Na⁺+K⁺-dependent ATPase activity during acclimation of the killifish Fundulus heteroclitus to salinity change. J. Exp. Zool. 202,179 -186.[CrossRef][Medline]

Towle, D. W., Rushton, M. E., Heidysch, D., Magnani, J. J., Rose, M. J., Amstutz, A., Jordan, M. K., Shearer, D. W. and Wu, W. S. (1997). Sodium-proton antiporter in the euryhaline crab Carcinus maenas: molecular cloning, expression and tissue distribution. J. Exp. Biol. 200,1003 -1014.[Abstract]

Towle, D. W., Paulsen, R. S., Weihrauch, D., Kordylewski, M., Salvador, C., Lignot, J.-H. and Spanings-Pierrot, C. (2001). Na⁺+K⁺-ATPase in gills of the blue crab Callinectes sapidus: cDNA sequencing and salinity-related expression of ${alpha}$ -subunit mRNA and protein. J. Exp. Biol. 204,4005 -4012.[Medline]

Wang, B., Li, F., Dong, B., Zhang, X., Zhang, C. and Xiang, J. (2006). Discovery of the genes in response to white spot syndrome virus (WSSV) infection in Fenneropenaeus chinensis through cDNA microarray. Mar. Biotechnol. 8, 491-500.[CrossRef][Medline]

Wanson, S. A., Péqueux, A. and Roer, R. D. (1984). Na regulation and Na⁺,K⁺-ATPase activity in the euryhaline fiddler crab Uca minax (La Conte). Comp. Biochem. Physiol. 79A,673 -678.

Weihrauch, D., Ziegler, A., Siebers, D. and Towle, D. W. (2001). Molecular characterization of V-type H⁺-ATPase (B-subunit) in gills of euryhaline crabs and its physiological role in osmoregulatory ion uptake. J. Exp. Biol. 204, 25-37.[Abstract]

Welcomme, L. and Devos, P. (1988). Cytochrome C oxidase and Na⁺-K⁺ ATPase activities in the anterior and posterior gills of the shore crab Carcinus maenas L. after adaptation to various salinities. Comp. Biochem. Physiol. 89B,339 -341.[CrossRef][Medline]

Wilkinson, M. G., Samuels, M., Takeda, T., Toone, W. M., Shieh, J. C., Toda, T., Millar, J. B. and Jones, N. (1996). The Atf1 transcription factor is a target for the Sty1 stress-activated MAP kinase pathway in fission yeast. Genes Dev. 10,2289 -2301.[Abstract/Free Full Text]

Yamazaki, K., Okamura, C., Ihara, T. and Yasumasu, I. (1997). Two types of Na⁺-K⁺-ATPase alpha subunit gene transcript in embryos of the sea urchin, Hemicentrotus pulcherrimus. Zool. Sci. 14,469 -473.[Medline]

Yu, H. Y., Nettikadan, S., Fambrough, D. M. and Takeyasu, K. (1996). Negative transcriptional regulation of the chicken Na⁺/K⁺-ATPase alpha 1-subunit gene. Biochim. Biophys. Acta 1309,239 -252.[Medline]

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