Altered Formation of Hemichannels and Gap Junction Channels Caused by C-Terminal Connexin-32 Mutations

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The Journal of Neuroscience, May 15, 1999, 19(10):3752-3760

Altered Formation of Hemichannels and Gap Junction Channels Caused by C-Terminal Connexin-32 Mutations
Carmen Castro¹, Juan M. Gómez-Hernandez¹, Kaisa Silander², and Luis C. Barrio¹
¹ Unidad de Neurología Experimental-Consejo Superior de Investigaciones Científicas, Departamento de Investigación, Hospital "Ramón y Cajal," 28034 Madrid, Spain, and ² Deparment of Medical Genetics, University of Turku, FIN-20520 Turku, Finland

  ABSTRACT

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Hexamers of connexins (Cxs) form hemichannels that dock tightly in series via their extracellular domains to give rise togap junction channels. Here we examined the ability of a varietyof C-terminal Cx32 mutations, most of which have been identifiedin X-linked Charcot-Marie-Tooth disease, to form hemichannelsand to complete gap junction channels using the Xenopus oocytesystem. First, we show that undocked wild-type Cx32 hemichannelsat the plasma membrane can be detected as opening channels activatedby depolarization. We have been able to estimate the efficiencyof assembly of complete channels by measuring the time-dependentincorporation of preformed hemichannels into gap junction channelsafter cell-to-cell contact. These data offer strong evidence thathemichannels are the direct precursors of gap junction channels.Of 11 Cx32 mutants tested, a group of 5 mutations prevented theformation of functional hemichannels at the cell surface, whereas4 mutations were fully able to form precursors but reduced theability of hemichannels to assemble into complete channels, and2 mutants formed channels normally. The data revealed that a minimumlength of human Cx32 including the residue Arg-215 is requiredfor the expression of hemichannels at the cell surface and thatthe efficiency of hemichannel incorporation into complete channelsdecreased gradually with the progressive shortening of the cytoplasmicC-terminaldomain.

Key words: connexin; voltage gating; gap junction channel formation; hereditary motor sensory neuropathy; X-linked Charcot-Marie-Tooth disease; Xenopus oocyte

  INTRODUCTION

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Gap junctions are clusters of intercellular channels that form adherent regions where the direct passage of ions and othersmall molecules between neighboring cells occurs (Revel and Karnovsky,1967; Gilula et al., 1982). Connexins (Cxs) are the structuralproteins of these intercellular channels in vertebrates, of which15 isotypes of this multigene family have been cloned so far inrodents, as well as several orthologs in other species (Bruzzoneet al., 1996). In human, mutations of the Cx32 gene were foundin X-linked forms of Charcot-Marie-Tooth disease (CMTX) (Bergoffenet al., 1993), a hereditary peripheral neuropathy that is characterizedby abnormally low nerve conduction and chronic weakness with progressivemuscular atrophy and sensory loss of the distalextremities.

Cx32 is thought to form gap junction channels between the adjacent folds at noncompact myelin (Bergoffen et al., 1993). Thesereflexive channels may act as an adhesive structure as well asconstituting a radial pathway for the rapid passage of ions, smallmetabolites, and second messenger molecules between adjacent cytoplasmiccompartments of the perinuclear and adaxonal regions of Schwanncells (Balice-Gordon et al., 1998). To date, >130 different CMTXmutations have been identified, and they are distributed throughoutall topological domains of the Cx32 molecule (Bone et al., 1997).

Attempts to explain the molecular and cellular mechanisms leading to the CMTX phenotype from the location and type of mutationhave been hampered by our limited knowledge concerning the molecularstructure and contribution of the various Cx32 domains to channelformation. It is currently accepted that the assembly of connexinsinto channels is a two-step process. First, connexins oligomerizeinto connexons or hemichannels in the intracellular compartmentbefore their transport to the plasma membrane (Musil and Goodenough,1993; Kumar et al., 1995), and then the hemichannels come in contactand dock with another hemichannel from a neighboring cell to formthe complete channel. Most of the events and molecular mechanismsinvolved in the successive stages of channel formation are currentlynot well understood. There is increasing evidence that hemichannelsare the immediate precursors of gap junction channels, but directproof of this is still not forthcoming. It is expected that duringthe process of channel formation hemichannels are closed untilthey dock with another hemichannel, inducing the newly formedchannel to open (Loewenstein et al., 1981; Chow and Young, 1987).However, the opening of solitary hemichannels in the plasma membranecan be induced by certain pharmacological manipulations (DeVriesand Schwartz, 1992; Li et al., 1996) or by membrane potentialdepolarization (Paul et al., 1991; Gupta et al., 1994; Ebiharaet al., 1995; Ebihara, 1996).

Here, we report that human Cx32 is also able to form solitary hemichannels that open on depolarization. Taking advantage ofour ability to detect functionally undocked hemichannels at thecell surface, we have characterized the normal process of theincorporation of hemichannels into complete channels and examinedthe specific stage of channel formation altered by several C-terminalCx32 mutants associated withCMTX.

  MATERIALS AND METHODS

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Construction of human Cx32 mutants. The human Cx32 (HCx32) cDNA (kindly provided by N. M. Kumar; Kumar and Gilula, 1986) containingthe complete coding region was inserted into the plasmid pBScMXT(Gupta et al., 1994) between the 5' and 3' flanking regions ofnoncoding Xenopus $beta$ -globin sequence to boost expression. EightHCx32 mutants found in patients with the X-linked form of Charcot-Marie-Toothdisease and two non-CMTX-related mutations were introduced intothe wild-type cDNA by PCR site-directed mutagenesis. To generatethe mutants, the following oligonucleotide primers were used:E208K (sense, 5'-CGCGACATTGAGGATGATGCAGAT-3'; antisense, 5'-AAGGTGGTGTACCTCATCATCCGG-3'),which introduced a new Nru restriction site; Y211stop [sense 5'-TAGACCCCAAGGCCTCTCTCTGCC-3'(stopTAG); antisense, 5'-GACCACCTCGGCCACATTGAGGAT-3'], with anew translationally silent XbaI site; R215W (sense 5'-TGGGCCTGTGCCCGCCGAGCCCAG-3';antisense, 5'-TATGATGAGGTACACCACCTCGGC-3'), with a new NdeI restrictionsite; R215Q (sense, 5'-CAGGCCTGTGCCCGCCGAGCC-3'; antisense, 5'-GATGATGAGGTACACCACCTCGG-3'),which created a new StuI site; R215stop [sense, 5'-TGATGCCACATACCAGGCAACCTG-3'(stopTGA); antisense, 5'-GATGATGAGGTACACCACCTCGG-3']; C217stop(sense, stopTAG; antisense, 5'-GGCCCGGATGATGAGGTACACCAC-3'); R220stop(sense, stopTGA; antisense, 5'-GCGGGCACAGGCCCGGATGATGAG-3'); R238H(sense, 5'-CCGGAATACAAGCAGAATGAGATC-3'; antisense, 5'-AGACAGGTGGTGGCCGAAGCCCGA-3'),with a new AccIII site; R265stop (sense, stopTAG; antisense, 5'-GCGCAGTATGTCTTTCAGGGAGCCAT-3');and S281stop (sense, stopTAG; antisense, 5'-GCAGCGGTCGCTCTTTTCAGCCAG-3').The PCR products were digested by DpnI endonuclease to eliminatethe template and with Pfu DNA polymerase (Stratagene, La Jolla,CA) to remove the bases extended onto the 3' ends before ligation.The whole coding region of the C280G mutation amplified from genomicDNA using primers 1F and 2R (Ionasescu et al., 1994) was directlyinserted into the EcoRV site of the pBScMXT vector. Mutants werescreened by size or restriction enzyme analysis and confirmedby DNA sequencing of the entire coding region on bothstrands.

In vitro transcription of cRNAs. Capped cRNAs were transcribed by T₃ RNA polymerase from 10 µg of SalI-linearized plasmid.The cRNA synthesis was performed under standard reaction conditions(protocol and reagents from Promega, Madison, WI) in the presenceof the cap analog m⁷G(5')ppp(5')G (Boehringer Mannheim, Mannheim, Germany). AfterDNase digestion and purification, cRNAs were quantified by absorbance(260 nm), and the proportion of full-length transcripts (>90%)was checked by agarose gelelectrophoresis.

Expression in Xenopus oocytes. Adult female Xenopus laevis frogs were purchased from Nasco (Fort Atkinson, WI), and oocyteswere prepared as previously described (Barrio et al., 1997). Oocytesin stages V and VI were co-injected with an antisense oligonucleotidedirected against Xenopus Cx38 mRNA to block endogenous expression(10 ng/oocyte; Barrio et al., 1991), and with the in vitro-transcribedcRNA of wild-type and CMTX mutants (0.1-0.5 µg/µl, 50 nl/oocyte).

Translation in oocytes. Seventy-two hours after RNA injection, oocytes were homogenized with lysis buffer (in mM: 5 Tris,5 EDTA, 5 EGTA, and 20 PMSF and 10 mg/ml leupeptin) and centrifugedto remove the yolk. Membranes were precipitated by centrifugation(100,000 × g, 30 min) after 30 min incubation in alkaline solution(20 mM NaOH). The membrane pellet was resuspended in loading buffer(25 mM Tris, 0.5% SDS, 18% glycerol, and 143 mM 2-mercaptoethanol).For each mutant, four oocyte equivalents per lane were loadedin a 4-20% Tris-glycine SDS-PAGE gel (Bio-Rad, Hercules, CA).After separation, proteins were transferred to nitrocellulosemembranes and visualized with 0.2% Ponceau S. Immunodetectionwas performed with the M12.13 antibody (Goodenough et al., 1988;Chemicon, Temecula, CA), which recognizes the cytoplasmic loopof Cx32. Specific bands were detected by enhanced chemiluminescence(ECL kit; Amersham, Buckinghamshire, England) following the instructionsof themanufacturer.

Macroscopic hemijunctional and junctional currents. Oocytes injected with the wild-type and mutated Cx32 cRNAs were recordedin ND96 medium (in mM: 96 NaCl, 2 KCl, 1 MgCl₂, 1.8 CaCl₂, and5 HEPES, pH 7.40) using microelectrodes of 0.5-1 M $Omega$ filled with2 M KCl, 10 mM EGTA, and 10 mM HEPES, pH 7.20. To explore thechannel-forming ability of mutated Cx32, the vitelline membranewas removed 24 hr after injection, and oocytes were paired tofacilitate the formation of cell-to-cell channels. The macroscopicjunctional currents (I_j) were measured and analyzed as previouslydescribed (Barrio et al., 1997). The transmembrane currents attributableto opening hemichannels (I_hj) were directly recorded under voltageclamp with two electrodes in isolated oocytes, and in the coupledpairs, the currents were calculated as I_hj = I_total $-$ I_j for eachcell of thepair.

Patch-clamp recordings. The patch-clamp experiments were performed according to standard techniques. Borosilicate glass pipettes(LE16; Dagan, Minneapolis, MN) of 1.5-4 M $Omega$ resistance were filledwith ND96 solution, and the bath solution was standard internalsolution (in mM: 100 KCl, 10 HEPES, and 10 EGTA); under theseconditions, the expected membrane potential of the oocyte wasnear zero, as confirmed by the lack of appreciable differencesin unitary conductance and the reversal potential of hemichannelsbetween cell-attached and inside-outside configurations. We usedan Axopatch 1D amplifier (Axon Instruments, Foster City, CA) connectedto a personal computer compatible through a Digi-Data (Jessup,MD) 1200 interface, and data acquisition and analysis were performedusing the pClamp 6. The currents filtered at 1 kHz were sampledat 2 and 20 kHz. Patch recordings in cell-attached and inside-outconfigurations were performed in oocytes for which positive expressionwas previously measured at the macroscopiclevel.

  RESULTS

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

We have evaluated the hemichannel- and channel-forming ability of 11 mutants lying between residues 208-283 of the HCx32 molecule.Nine of these mutations have been implicated in CMTX; their locationis illustrated in Figure 1A. The group of nonsense CMTX mutationsleading to truncated proteins are as follows: Y211stop (Tan etal., 1996), C217stop (Ionasescu et al., 1994, 1996), R220stop(Fairweather at al., 1994; Bone et al., 1995; Ionasescu et al.,1996), and S281stop (Nelis et al., 1997). An additional truncationgenerated by a 29-bp deletion beginning at amino acid 265, whichproduces a stop codon directly after position 265 has also beentested (R265stop; Ionasescu et al., 1996). Furthermore, the groupof missense CMTX mutations analyzed includes E208K (Fairweatheret al., 1994), R215W (Fairweather et al., 1994; Ressot et al.,1996; Bort et al., 1997), R238H (Nelis et al., 1997) and C280G,not previously published. The novel C280G mutation was detectedin one Hungarian family by direct sequencing of the Cx32 gene(see methods in Silander et al., 1997), a 30-year-old male beingdiagnosed with CMT based on electrophysiological study and nervebiopsy findings. His subjectively healthy mother was found tocarry the mutation and showed decreased nerve conduction. Themutation was not present in three unaffected family members (fatherand two maternal cousins) and 100 Finnish controls.

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Figure 1. Hemichannel- and channel-forming ability of the CMTX mutants. A, Diagrams of the topological domains of HCx32 molecule and the location of the nine CMTX mutations and two nonrelated CMTX mutants, R215stop and R215Q, tested. M1, M4, Transmembrane domains; E1, E2, extracellular loops; CL, cytoplasmic loop; NT, N terminal; CT, C terminal. B, Sample records of macroscopic transmembrane currents induced by depolarizations from $-$ 40 to +120 mV by increments of 20 mV and of 10 sec duration in isolated oocytes expressing the wild-type HCx32 and mutants. Depolarizations of +40 mV or greater induced slowly activating outward currents, which became larger as higher positive potentials were applied in oocytes expressing HCx32. Currents became inward and declined with a slow time course when the potentials returned to $-$ 40 mV. The induction of large currents with these unusual characteristics suggested the presence of Cx32 hemichannels preformed in the plasma membrane, which were normally closed at resting potentials and that open with depolarization (also see single channel recordings in Fig. 2). A group of mutants, E208K, Y211stop, R215stop, R215W, and R215Q, did not show detectable levels of hemichannels at the cell surface, whereas the oocytes expressing the C217stop, R220stop, R238H, R265stop, C280G, and S281stop mutants developed large hemichannel currents. C, Percentage of coupling in oocytes induced between nonsense (top) and missense (bottom) mutants relative to wild-type pairs. Coupling values are from the experiments in Figure 4. Nondetectable levels of coupling (NC) were found in pairs expressing the E208K, Y211stop, R215stop, R215W, and R215Q mutants. The C217stop, R220stop, R265stop, and S281stop mutants induced lower levels of coupling, whereas the R238H and C280G showed similar coupling to wild-type pairs. Asterisks indicate t test values that differ statistically (*p < 0.05; **p < 0.001).

Hemichannel-forming ability of C-terminal CTMX mutants

It is currently accepted that the first step leading to channel formation commences with the synthesis of connexins, theircorrect insertion into the membrane, and their hexameric assemblyinto connexons that are targeted and incorporate as hemichannelsin the plasma membrane. To evaluate the presence of preformedhemichannels at the cell surface, unpaired Xenopus oocytes expressingwild-type HCx32 and C-terminal mutants (Fig. 1B) were voltage-clampedto a holding potential of $-$ 40 mV, and positive pulses were appliedup to +120 mV depolarizations. In wild-type cells, macroscopicrecordings showed typically slow activating outward currents detectableat depolarizations of +40 mV or greater and larger currents atgreater positive voltages. Currents became inward and declinedwith a slow time course when the potentials returned to $-$ 40 mV.In contrast, oocytes injected exclusively with the antisense oligonucleotidedirected against the endogenous connexin component (Barrio etal., 1991) did not exhibit this type of current. Thus, the inductionof large currents with these unusual characteristics suggestedthe presence of Cx32 hemichannels preformed in the plasma membrane,which were normally closed at resting potentials and that openwith depolarization. Cell-attached single-channel patch-clamprecordings from oocytes expressing human Cx32 allowed us to confirmthe presence of opening hemichannels (Fig. 2A), which displayedproperties consistent with those observed at the macroscopic level.With smaller depolarizations, the first hemichannel openings typicallyoccurred after a long latency after the pulse onset, in agreementwith the delayed activation of macroscopic currents. With largerpulses, latencies shorted, and the open time duration and numberof hemichannels open increased progressively. The unitary currentsbecame inward when returning to the holding potential of $-$ 40 mV,and the hemichannels showed a characteristic flickering activitywith frequent and recurrent transitions between the open and fullyclosed states before actually closing. This activity was consistentwith the slow kinetics of the macroscopic tail currents. Patchescontaining one or two hemichannels were selected to study single-channelproperties. The HCx32 hemichannels recorded in physiological solutionsshowed a main open state conductance of ~17 pS and fast transitions(<1-2 msec) between the main open and fully closed states. Inaddition, transitions to at least two subconductance states of12 and 4 pS were often observed (Fig. 2B). Unitary currents associatedwith the main open state did not rectify into the voltage rangeexplored, from $-$ 40 to +120 mV, and reversed near $-$ 10 mV (Fig.3A). These properties of HCx32 hemichannels differ markedly fromthose previously reported for the Cx46 hemichannels (Trexler etal., 1996), indicating that the unitary characteristics of differenthemichannels depend on their connexin composition.

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Figure 2. Cell-attached single-channel recordings of HCx32 hemichannels. A, Depolarization of +40 mV and greater induced opening events whose properties are consistent with those observed at macroscopic level in Figure 1B. Unitary currents became inward returning to a holding potential of $-$ 40 mV and exhibited a characteristic bursting activity before complete closure. B, Selected patch records containing two open hemichannels at +60 mV. Hemichannel activity showed fast transitions between closed (C) and main open (O) states of 17 pS and less frequently to, at least, two subconductance states (S₁ and S₂) of 12 and 4 pS.

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Figure 3. Properties of functional CMTX hemichannels. A, Unitary properties of C217stop and wild-type hemichannels. Selected single-channel recordings in cell-attached configuration of patches containing two open hemichannels at +80 mV show fast current transitions between closed and main open states and less frequently to subconductance states (top). The unitary current-voltage relationships of the main open state for wild-type and C217stop hemichannels were linear from +120 to $-$ 40 mV, and the currents reversed near $-$ 5 mV (bottom). The unitary conductance values calculated from the slope of the linear fits were of 16.9 ± 0.4 and 17.5 ± 1.0 pS for wild-type and C217stop hemichannels, respectively. Each point represents mean values of 12-16 patches from different oocytes. Error bars indicate SEM. B, Voltage dependence and limiting voltage sensitivity (inset) of hemichannels comprising wild-type HCx32 and the C217stop and R220stop mutants. Hemijunctional conductance (G_hj) measured at the end of pulses was normalized relative to the value for +120 mV pulse. Note the progressive shift of the threshold of activation (inset) and conductance-voltage curves toward higher positive potentials with the shortening of the C-terminal domain. Each point is the mean value of 10 measurements. Error bars indicate SEM.

All HCx32 mutants were efficiently translated in oocytes and gave rise to proteins of the expected sizes, as revealed by Westernblot analysis (data not shown). Those oocytes expressing mutantslocated at more distal regions, C217stop, R220stop, R238H, R265stop,C280G, and S281stop, developed large hemijunctional conductanceswhose levels were comparable to those found in the wild-type Cx32oocytes. In contrast, oocytes injected with the E208K and Y211stopmutants did not show detectable levels of opening hemichannelsin the voltage range explored (Fig. 1B). We also constructed anonrelated CMTX mutant with a premature stop codon at position215, which was incapable of forming functional hemichannels inthe plasma membrane. These results indicate that there is a minimumlength of the carboxyl tail needed to retain hemichannel-formingability at the cell surface. In this context, we observed thatwhen Arg-215 was substituted by Trp in the full-length Cx32 (R215W),the ability to form hemichannels was completely impaired. Becausethe hydrophobic nature could account for R215W effects, we testedthe R215Q substitution, which also led to a complete loss of function.Thus, we concluded that the presence of Arg-215 is required forCx32 to retain the ability to form functional hemichannels, afunction that could not be rescued by the other four positivelycharged amino acids, Arg-219, -220, -223, and -224.

The C-terminal mutations did not change the unitary properties of hemichannels, because even in the case of the shortest mutantwith hemichannel function, C217stop, its unitary conductance inthe main open state was close to ~17 pS; moreover, currents revertednear $-$ 5 mV and behaved linearly from $-$ 40 to +120 mV (Fig. 3A).However, the C217stop, R220stop, and R265stop hemichannels exhibitednovel voltage-gating properties at macroscopic levels (Fig. 3B).The activation of wild-type hemichannels was detectable at depolarizationsof +40 mV or greater, whereas the threshold for the R265stop andR220stop hemichannels increased to +50-60 mV, and that for C217stophemichannels increased to depolarizations of +80 mV or greater.In parallel, the curves of activation shifted progressively towardhigher positive potentials. The voltage-gating properties of R238Hand C280G mutants were as those of the wild-typehemichannels.

Gap junction channel-forming ability of C-terminal CTMX mutants

Making hemichannels is only half the process in cell-to-cell channel formation. The final stage of channel formation involvesthe aligning, recognition and docking of hemichannels in adjacentcells via their extracellular domains (Dahl et al., 1991, 1994;Meyer et al., 1992). The formation of the channel is completedby the final gating of the two closed hemichannels to an openconfiguration. Channel formation between paired cells was estimatedfrom the development of coupling after cell-to-cell contact bymeasuring the macroscopic junctional conductance. The mutationslocated closest to the cytoplasmic-membrane boundary, mutantsR215W, R215Q, R215stop, Y211stop, and E208K, produced a completeloss in the ability to form complete channels (Fig. 1C). A secondgroup of mutations that included the truncations C217stop, R220stopand R265stop, and S281stop developed very low, moderate, or almostnormal levels of junctional conductance, respectively, and a thirdgroup formed by the R238H and C280G mutants showed similar levelsof coupling to the wild-type HCx32 (Fig. 1C). Thus, it appearsthat only those mutants that induced the expression of functionalhemichannels were also able to form complete intercellular channelsand that the effects of the mutations depended on the combinedaction of their location and the type of mutation. The removalof the last three amino acids of the carboxyl tail, S281stop,or the C280G substitution had little or no effect on the channel-formingability. The additional deletion of the C-terminal tail up topositions 264 and 219 markedly reduced the coupling to nearlyhalf the value of the wild type, whereas the R238H substitutionin this region did not alter the channel-forming ability. TheC217stop mutant, which has a shorter C-terminal tail, in whichonly four extra amino acids were deleted with respect to the R220stopmutant, still retained the ability to form channels, but the efficiencyto induce coupling was reduced by >95%. These results indicatethat although the majority of the C-terminal domain is not a structuralrequirement to form gap junction channels, this domain plays acritical role determining the efficiency of channelformation.

A discrepancy was observed with the mutants C217stop, R220stop, and R265stop between the large amount of channel precursorsand the low levels of coupling induced. To evaluate the channel-formingefficiency of those mutants with respect to the wild-type Cx32,the cRNA concentrations injected were empirically adjusted tothose that induced similar levels of macroscopic hemijunctionalconductance (Fig. 4A, insets). Under these conditions, the temporalpattern of mutated hemichannels at the cell surface of unpairedoocytes expressing wild-type and mutated Cx32 overlapped, indicatingthat they underwent similar processing as wild-type ones. Thetime course of hemichannel expression at the cell surface wascharacterized by a delay of 6-12 hr after cRNA injection untilmacroscopic currents attributable to hemichannel openings becamedetectable in the plasma membrane. This delay probably reflectsthe time required for connexin synthesis, assembly into hemichannels,and transport to plasma membrane. Hemichannels accumulated rapidly,reached peak values between 48 and 72 hr, and then declined slowlyand progressively with time. In the same experiments, the setof paired oocytes expressing the S281stop, R265stop, R220stop,and C217stop mutants developed a lower degree of coupling, 89,44, 37, and 5% of the wild-type pairs, respectively. Thus, theC217stop mutant is an example of a fully functional mutation withrespect to the formation of hemichannels but with an almost completeinability to induce functional channels. The lower coupling inducedcould be accounted for by a reduction in the assembly of precursorsinto gap junction channels, or alternatively, it may reflect thefailure of newly formed channels to achieve the final open conformation.To discern between these two possibilities, we used an experimentalparadigm in which the pool size of solitary hemichannels in bothcells of each pair was monitored in parallel with channel formationwhen oocytes were brought into contact manually and compared withthe amount of hemichannels expressed in oocytes that remainedisolated (Fig. 4). The time course of wild-type channel formationwas approximately sigmoidal, with a latency of minutes or a fewhours until coupling became detectable (>10 nS). Coupling waspreceded by a slow increment of junctional conductance duringthe first 24 hr after pairing and was followed by a rapidly increasingphase (48-72 hr after pairing) during which the rate of channelformation accelerated progressively. During the last phase ofcoupling (72-144 hr after pairing), coincident with the decreasingphase of hemichannel expression, the junctional conductance increasedslowly (Fig. 4A, top and bottom). Thus, in contrast to the poolof undocked hemichannels whose expression declined with time,the hemichannels assembled into complete gap junction channelsseemed to constitute more stable structures, because the poolof newly formed channels tended to increase progressively in nascentgap junctions over the same time scale. These results also revealthat the formation of junctional channels is favored over thepersistence of solitary hemichannels, suggesting that once hemichannelsare assembled, the undocking process is less probable or doesnot occur. Our observation that the hemichannel and complete channelundergo different rates of removal at the cell surface of Xenopusoocytes is consistent with the recent observation in which thedegree of dye coupling does not decrease significantly when 85%of connexin staining disappeared, with a half life of ~1 hr, fromapposed mammalian cell membranes (Laing et al., 1997).

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Figure 4. Efficiency of the CMTX hemichannels to assemble into intercellular channels. A, To evaluate the efficiency of assembly, the wild-type and mutated cRNA concentrations were empirically adjusted to those that induced similar levels of hemijunctional conductance (insets). The time course of channel formation of the homotypic pairs expressing the C217stop and R220stop (top) and R265stop (bottom) mutants indicates slower coupling, reaching lower levels than the respective control wild types. The reduction in coupling was small for S281stop (bottom), moderate in the case of R265stop and R220stop, and marked for C217stop. The deficient channel formation induced by C217stop and R265stop alone could be rescued partially in heterotypic combinations by the wild-type Cx32 hemichannels (broken lines). B, Measurement of the hemichannel pools in isolated and paired oocytes injected with the wild-type and C217stop, R220stop, and R265stop mutants. Data are from the experiments in A. In the paired oocytes expressing the mutants there was an excess of solitary hemichannels relative to those found in the wild-type Cx32 pairs, revealing an inefficient assembly of hemichannels into complete channels. Each point in A and B represents mean values of 20-25 measurements from four experiments. Error bars indicate SEM. C, Percentage of hemichannels incorporated into complete channels. The amount of incorporation was calculated as the difference of hemijunctional conductances between isolated and paired oocytes, and in case of the mutants their values were normalized relative to the percentage of wild-type incorporation. The reduction was consistent with the lower levels of coupling induced by the C217stop, R220stop, and R265stop mutants. h.a.i., Hours after injection; g_j, junctional conductance; g_hj, hemijunctional conductance.

According to the assumption that newly formed channels were formed by the progressive docking of preformed hemichannels contributedby each cell of a pair, the size of the hemichannel pools measuredin both cells of the pair decreased relative to that found inthe unpaired oocytes (Fig. 4B), the reduction being similar ineach cell of the pair, and its time course was parallel to thecoupling development. This reduction was not complete, becausea certain amount of solitary hemichannels remained at the cellsurfaces of paired oocytes when longer pairing times were analyzed.The percentage of hemichannels incorporated into complete channelswas estimated as the difference between the macroscopic hemijunctionalconductance in paired oocytes relative to that found in parentisolated oocytes. It varied between 30 and 60% depending on thebatches of oocytes used and, more importantly, on the level ofprecursor expression, because less incorporation occurred at lowerlevels of hemichannel expression (data not shown). The percentageof incorporation relative to the total number of hemichannelsdelivered to the plasma membrane would necessarily be smaller,because approximately half of the hemichannel pool was removedfrom the membrane before they could bedocked.

The pool of channel precursors that remained as undocked hemichannels in paired oocytes was abnormally large for CMTX mutantsthat induced low levels of coupling (Fig. 4B). The percentageof hemichannels incorporated into complete channels also decreasedrelative to that of wild-type Cx32 by up to 58 and 41%, respectively,in the case of the R265stop and R220stop but only 3.4% for C217stop(Fig. 4C). This reduced incorporation to channels is consistentwith the lower levels of coupling previously measured, indicatingthat this group of mutants altered the assembly process of twohemichannels into an intercellular channel. Interestingly, theinefficient assembly could be partially rescued by wild-type hemichannelswhen oocytes that expressed wild-type HCx32 were paired with thoseexpressing the C217stop or R265stop mutants (Fig. 4A, broken lines).These heterotypic combinations favored the development of couplingrelative to the combinations of mutants alone, although this rescueeffect was slight in the case of the hybrid junctions with theC217stop mutant and more pronounced in combination with the R265stophemichannels. These data indicate that channel assembly is a cooperativeprocess, the efficiency of which results from the combined actionof both contributinghemichannels.

  DISCUSSION

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ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

Assembly of preformed hemichannels into gap junction channels

Our data provide electrophysiological evidence that human Cx32 forms hemichannels at the cell surface and that such hemichannelsare the immediate precursors of the gap junction channels. Theefficiency of the processes leading to the channel formation isonly just beginning to be understood. The efficiency of connexinassembly into hemichannels reported in vivo and in vitro is aslow as ~20% (Musil and Goodenough, 1993; Falk et al., 1997), similarto that for other ionic channels (for review, see Green and Millar,1995). In the present study, when the efficiency of hemichannelassembly into complete channels was first determined, it appearedto represent a similarly inefficient process, considering jointlythe continuous removal of unpaired hemichannels already presentat the cell surface and the percentage of hemichannels incorporatedinto complete channels. Taken together, it may be that only 5%of HCx32 is incorporated into gap junction channels. Additionalexperimentation will be required to confirm whether the low efficiencyof hemichannel assembly is a common feature among different connexinsand different celltypes.

In this and previous studies of nascent gap junctions using induced cell pairs, the development of coupling follows a characteristicsigmoidal time course (Dahl et al., 1991; Valiunas et al., 1997).Channel formation first proceeds slowly and later increases rapidlyuntil reaching saturating values. This indicates that gap junctionformation is an autofacilitated process rather than a simple additionof one channel at a time in an independent manner. Our abilityto quantitate the pool of channel precursors allowed us to observethat the initial slow rate of channel formation occurs even whenlarge amounts of preformed hemichannels are already present atthe cell surface of both contributing cells. Thus, the formationof the first complete channels of nascent gap junctions may beby itself a limiting factor in coupling development. Accordingly,the CMTX mutants with a limited ability to form complete channelsshowed a slower rate of channel formation during longer periods(Fig. 4A).

Role of the C-terminal domain in the hemichannel and channel formation

In our studies of distinct Cx32 C-terminal mutants, two types of effects were found depending on the location and type ofmutation (Table 1). Five mutations (E208K, Y211stop, R215W, R215Q,and R215stop) prevented the formation of functional hemichannelsat the cell surface, whereas four mutants (C217stop, R220stop,R265stop, and S281stop) reduced the ability of hemichannels toassemble into complete channels. Conversely, the R238H and C280Gmutants were fully capable of forming functional intercellularchannels. Taken together these data indicate that a minimum lengthof the protein, which includes the presence of Glu-208 and Arg-215residues, is a structural requirement for the formation of functionalhemichannels at the cell surface. Accordingly, the cellular localizationof the E208K mutant transfected into mammalian cells was entirelycytoplasmatic (Deschênes et al., 1997), and R215W staining atadjacent cell surfaces was greatly reduced (Omari et al., 1996),indicating that trafficking to the plasma membrane is altered.However, the extrapolation of these results to Xenopus oocytesmight be limited given the differences in subcellular locationof R142W and E186K mutants reported between the two cell types(Bruzzone et al., 1994; Deschênes et al., 1997).


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Table 1. Hemichannel- and channel-forming ability of C-terminal Cx32 mutants associated with CMTX expressed in Xenopus oocytes

Our findings from the truncated C-terminal CMTX mutants are consistent with previous results obtained from the rat Cx43 (Durhamet al., 1992) and rat Cx32 (Rabadan-Diehl et al., 1994). In thepresent study, we could ascribe the complete loss of channel formationto the absence of functional hemichannels at the cell surface,whereas the gradual decrease of coupling associated with the progressiveshortening of the carboxyl tail length can be accounted for bya defect in the assembly of mutated hemichannels into completechannels (Table 1). The role that the carboxyl domain plays infacilitating assembly is intriguing. It has been well establishedthat the binding site between hemichannels is complex and involvesseveral segments of the two extracellular domains (Dahl et al.,1994; White et al., 1994; Haubrich et al., 1996). There is evidencethat hemichannel binding could involve hydrophobic interactions,hydrogen bonds, and ionic attractions (Goodenough and Gilula,1974; Manjunath et al., 1984; Ghoshroy et al., 1995), and thatmultiple weak bonds can contribute to the stability of two hemichannelsdocking. Based on ultrastructural studies and consistent withthe evidence of a disulfide-bonded $beta$ -sheet provided by scanningcysteine mutagenesis studies (Foote et al., 1998), the extracellularsurface of hemichannels forms six protrusions (Hoh et al., 1991,1993; Perkins et al., 1997). This has led to the proposal thata "lock and key" mechanism mediates docking (Perkins et al., 1998).Because each extracellular protrusion may also include an extensionof the intramembranous $alpha$ -helical structure (Tibbitts et al., 1990),most likely contributed to by the third and fourth transmembranesegments as the predicted lengths postulated to span the bilayerare clearly excessive, it is possible that the mutations suchas C217stop and R220stop located close to the inner membrane-cytoplasmicboundary may induce a conformational change of the binding surface,which may reduce the strength and/or affinity of binding betweenhemichannels. Such a structural change seems less possible inthe case of the C-terminal truncations, because R265stop is locatedmore distally. An alternative explanation is that the C-terminaldomain might be involved in a global conformational change ofmolecule needed to stabilize the assembly between two hemichannels.The assumption that there is an "induced fit" rather than a lockand key mechanism governing hemichannel-hemichannel binding isspeculative at this time, but it might explain the striking correlationobserved in this study between the gradual reduction of hemichannelincorporation into complete channels (Fig. 4C) and the progressiveincrements of the voltage needed to induce hemichannel opening(Fig. 3B). We interpret this linkage between both processes asattributable to the existence of a common gate for voltage andchemical binding; even the structure-function determinants ofboth gatings must not be the same. Based on the novel voltage-gatingproperties of mutated hemichannels (C217stop, R220stop, and R265stop),it is conceivable that the C-terminal truncations may cause conformationalchanges in the molecule, which would affect the energy barrierprofile of the gate in a manner that increases the activationenergy for opening. If this is so, we would also expect a limitedability of hemichannels to open by the chemical mechanism and,consequently, a reduction in the efficiency of hemichannel assemblyinto gap junctionchannels.

Cx32 mutations and CMTX disease

As more becomes known about CMTX mutants, it is evident that a greater diversity of pathomechanisms seems to cause the disease.To date, 27 mutants of the 160 mutations identified in CMTX patientshave been analyzed using exogenous expression systems, includingthe 9 mutants described here (Bruzzone et al., 1994; Rabadan-Diehlet al., 1994; Omari et al., 1996; Deschênes et al., 1997; Ohet al., 1997; Ressot et al., 1998). Twelve mutants have been reportedas null mutations, whereas 15 mutants still produce functionalintercellular channels, although their efficiency in most caseshas not been addressed. In our series, at least four of six functionalmutants have a limited ability to form complete channels (Table1). Mutations may also impair channel function, such as has beenreported in the case of two mutants that reduce the junctionalpermeability or open probability (Oh et al., 1997), and for thegroup of mutants that exhibit altered voltage- and pH-gating properties(Ressot et al., 1998). In this context, we found that five ofsix functional junctions (C217stop, R220stop, R238H, R265stop,and S281stop) showed novel voltage-gating properties. The effectswere not pronounced, but, interestingly, the changes were mutation-specific.

The severity of the CMTX clinical phenotype seems to correlate with the location and type of mutation in the Cx32 gene (Ionasescuet al., 1996; Deschênes et al., 1997), although strict correlationsbetween genotype and clinical phenotype are still to be established.In this context, our results suggest that different mutationscould lead to severe phenotypes by altering different mechanisms.The severe phenotype of E208K (Deschênes et al., 1997) and Y211stop(Hahn et al., 1990) mutants may be caused by the complete lossof channel function. The possibility of dominant negative interactionswith other myelin proteins has also been proposed based on thedefective trafficking of E208K to the cell surface (Deschêneset al., 1997). In the case of the C217stop, R220stop, and R265stopmutants, which form hemichannels whose assembly is inefficient,they may cause a severe clinical phenotype (Ionasescu et al.,1996) by limiting channel formation or owing to an excess of solitaryhemichannels, which could adversely affect cell viability if theywere to open. The presence of open hemichannels may have a deleteriouseffect, as has been demonstrated in oocytes overexpressing Cx46,in which they induced swelling and cell lysis because they arenormally open at resting membrane potential (Paul et al., 1991).In the case of HCx32 hemichannels, opening on depolarization isunlikely given the high positive voltage required, but the possibilitythat opening may be induced by other physiological agents is presentlyunderinvestigation.

  FOOTNOTES

Received Dec. 11, 1998; revised Feb. 19, 1999; accepted March 9, 1999.

This research was supported by Fondo de Investigaciones Sanitarias (FIS) Grant 95/0643, Fundación "la Caixa" Grant 97/123-00,and Ministerio de Educación y Cultura Grant PM97-0021 (to L.C.B.).L.C.B. is member of the European Charcot-Marie-Tooth Consortium(BIOMED2 Grant CT961614). J.M.G.-H. is a postdoctoral fellow ofthe Comunidad Autónoma de Madrid. C.C. is the recipient of anFIS fellowship. We are grateful to N. M. Kumar for providing theHCx32 cDNA. We acknowledge the cooperation of the Hungarian familyin this study and Dr. V. Karcagi for providing data on the patients.We also thank R. Barquero for invaluable technical assistancewith the oocyteexperiments.
Correspondence should be addressed to Dr. Luis C. Barrio, Departamento de Investigación, Unidad de Neurología Experimental-ConsejoSuperior de Investigaciones Científicas, Hospital "Ramón y Cajal,"Carretera de Colmenar km 9.1, 28034 Madrid,Spain.

  REFERENCES

TOP
ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
REFERENCES

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