HOME HELP FEEDBACK SUBSCRIPTIONS ARCHIVE SEARCH TABLE OF CONTENTS		QUICK SEARCH:   [advanced] Author: Keyword(s): Year:  Vol:  Page:

This Article Abstract Full Text (PDF) Submit a response Alert me when this article is cited Alert me when eLetters are posted Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via Google Scholar Google Scholar Articles by Xu, X. Articles by Ebihara, L. Search for Related Content PubMed PubMed Citation Articles by Xu, X. Articles by Ebihara, L.

Characterization of a Mouse Cx50 Mutation Associated with the No2 Mouse Cataract

From the Department of Physiology and Biophysics, FUHS/The Chicago Medical School, North Chicago, Ilinois.

	Abstract

Top Abstract Introduction Materials and Methods Results Discussion References

 
PURPOSE. Recently, a missense mutation in the mouse connexin 50 (Cx50) gene has been associated with the nuclear opacity 2 (No2) mouse cataract. This missense mutation (D47A) resulted in an aspartate-to-alanine substitution at amino acid position 47 in the first extracellular domain of Cx50. To better understand the role of Cx50 in the pathogenesis of congenital cataract, the functional consequences of the D47A mutation in the Xenopus oocyte expression system were studied.

METHODS. D47A was constructed using polymerase chain reaction (PCR) mutagenesis. Xenopus oocytes were injected with in vitro transcribed cRNA encoding wild-type mouse Cx50 (Cx50wt), wild-type rat Cx46 (Cx46wt), D47A, or combinations of wild-type and mutant connexins. The oocytes were then devitellinized and paired. Gap junctional conductance (G_j) was measured using a dual two-microelectrode voltage-clamp technique.

RESULTS. Homotypic oocyte pairs expressing wild-type Cx50 or Cx46 were well coupled. In contrast, oocytes injected with D47A cRNA did not form gap junctional channels when paired homotypically. To test whether the D47A mutation could interact with wild-type connexins in a dominant negative manner, oocytes were injected with equal amounts of mutant and wild-type connexin cRNA, mimicking the heterozygous condition. Expression of D47A did not inhibit the development of junctional conductance in paired oocytes induced by wild-type Cx50 or Cx46.

CONCLUSIONS. These results indicate that the D47A mutation acts as a loss-of-function mutation without strong dominant inhibition. In No2 mice, the mutation would be predicted to result in a reduction in intercellular communication, leading to cataractogenesis. It may also cause other qualitative changes such as a change in permeability for small molecules.

	Introduction

Top Abstract Introduction Materials and Methods Results Discussion References

 
Gap junction channels are intercellular pathways between adjacent cells for the exchange of ions and metabolites smaller than 1 kDa.¹ The gap junction channel is made of two hemichannels, each contributed separately by two adjoining cells. The hemichannels are composed of six subunits called connexins. The connexins belong to a multigene family composed of at least 14 members.¹ Gap junctional channels are defined as homotypic when they contain a single type of connexin and heterotypic when each hemichannel of the pair is composed of a different connexin subtype. Heteromeric channels are those in which the hemichannels are composed of more than one connexin type.

The lens is an avascular organ that is highly dependent on intercellular communication for volume regulation and metabolic homeostasis.² Three connexins have been identified in the rodent lens: Cx43, Cx46, and Cx50.^{3 4 5} Mouse connexin 50 (mCx50) is expressed only in the lens, where it forms gap junctional channels between fiber cells.⁴ Connexin 46 is also found in lens fiber–fiber gap junctions, whereas connexin 43 is expressed in lens epithelial cells.³

Mutations in connexins have been linked to several genetic diseases including X-linked Charcot–Marie–Tooth disease (CMTX), a demyelinating peripheral neuropathy that is associated with mutations in Cx32^{6 7 8} ; hereditary nonsyndromic deafness, which is associated with mutations in Cx26⁹ ; and visceroatrial heterotaxia syndromes, which are associated with mutations in Cx43.¹⁰ Recently, a missense mutation in the mouse connexin 50 gene (Gja8) has been associated with the nuclear opacity 2 (No2) mouse cataract, a congenital hereditary bilateral cataract that is inherited in a semidominant manner.^{11 12} This missense mutation results in a substitution of aspartic acid-to-alanine at amino acid position 47 in the first putative extracellular domain of Cx50. To understand better the role of Cx50 in the pathogenesis of congenital cataract, we studied the functional consequences of the Cx50D47A mutation by testing its ability to induce gap junctional coupling between paired oocytes.

	Materials and Methods

Top Abstract Introduction Materials and Methods Results Discussion References

 
Mutagenesis
cDNAs encoding mouse Cx50 and rat Cx46 in the pSP64TII vector¹³ were provided by Thomas W. White and Daniel A. Goodenough (Harvard University, Boston, MA). To generate Cx50D47A, two primers corresponding to adjacent regions in the E1 domain of Cx50 were synthesized. The sense primer, 5'-CTGAGCAATCTGATTTTGTATGCAACACC-3', corresponding to nucleotides from 406 to 434, contained nucleotides encoding amino acid 47 to 56 of Cx50, with nucleotide 406 changed from A to C, resulting in the conversion of aspartic acid 47 to alanine. The antisense primer, 5'-CGCCCCACACAAACTCCGCT-3', corresponding to nucleotides from 405 to 386, corresponds to amino acids 40 to 47 of Cx50. Cx50 in the SP64T vector was amplified using a commercial kit (LA PCR; Takara Shuzo, Ostsu, Japan) according to the manufacturer’s protocol. The polymerase chain reaction (PCR) conditions were as follows: 1 minute at 94°C; 25 cycles at 98°C for 20 seconds and 68°C for 10 minutes; and 1 cycle at 72°C for 10 minutes. The PCR-amplified product was digested with the restriction enzyme, DpnI, to select against the parental, nonreplicated DNA.¹⁴ Subsequently, the PCR-amplified product was purified with a PCR purification kit (QIAquick; Qiagen, Chatsworth, CA), polished with a PCR polishing kit (Stratagene, La Jolla, CA), and ligated to itself to generate Cx50D47A SP64T. The mutant construct was sequenced to ensure that PCR amplification did not introduce any new mutations (DNA Sequencing Facility, Iowa State University, Ames, IA). The recombinant plasmid DNA was linearized with the restriction enzyme, SalI. cRNAs were in vitro transcribed with SP6 polymerase (mMessage mMachine kit; Ambion, Austin, TX) following the manufacturer’s protocol. The transcripts were purified on a G-50 Sephadex column (Boehringer Mannheim, Indianapolis, IN) to remove unincorporated rNTPs, precipitated with isopropanol, and resuspended in diethyl pyrocarbonate–treated water. The cRNA was quantitated by measuring the absorbance at 260 nm and stored as 3-µl aliquots at –80°C.

Preparation of Xenopus Oocytes
Female Xenopus laevis was anesthetized, and a partial ovariectomy was performed. The frogs were maintained and treated in accordance with National Institutes of Health guidelines and with the ARVO Statement for Use of Animals in Ophthalmic and Vision Research. The oocytes were treated with 10 mg/ml collagenase type IA (Sigma, St. Louis, MO) for 20 minutes, manually defolliculated, and injected with an oligonucleotide antisense to endogenous Cx38, as previously described.¹⁵ The oocytes were then injected with 3 to 4 ng cRNA for mouse Cx50, mouse Cx50D47A, or rat Cx46, either alone or in combination, and allowed to incubate for an additional 6 to 48 hours. Then the oocytes were devitellinized and paired as previously described.¹⁶ Electrophysiological measurements were performed 6 to 18 hours after pairing.

Western Blot Analysis of Connexin Proteins
Plasma membrane–enriched preparations of Xenopus oocytes were prepared as previously described.^{3 17} The proteins were resolved on a sodium dodecyl sulfate–containing 9% polyacrylamide gel and transferred to nitrocellulose. The western blots were probed with the anti-Cx50 monoclonal antibody 6-4-B2-C6 (kindly provided by Viviana Berthoud and Eric Beyer, University of Chicago, IL).¹⁸ The primary antibody was detected with alkaline phosphatase–conjugated goat anti-mouse Ig (Boehringer–Mannheim, Indianapolis, IN).

Electrophysiological Measurements and Analysis
Dual two-microelectrode voltage-clamp recordings of gap junctional channels were performed (Axoclamp 2A and a Geneclamp 500 amplifier; Axon Instruments, Foster City, CA). The current and voltage electrodes were filled with 3 M KCl and had resistances of 0.1 to 0.5 M. The tips of the electrodes were back filled with 1% agar in 3 M KCl to prevent KCl from leaking out of the electrodes and damaging the oocytes. Data acquisition and analysis were as performed (Pentium computer equipped with a TL-1 labmaster board and Pclamp6 software; Axon Instruments, Austin, Texas). Currents were filtered at 50 Hz using a four-pole Bessel filter. All experiments were performed at room temperature (22°C–24°C). For simple measurement of gap junctional conductance, both cells of the pair were initially voltage clamped to –40 mV and a 5- to 10-mV pulse was applied to one cell. Under these conditions, the change in current recorded in the second cell would be equal in magnitude and opposite in polarity to the current flowing through the gap junction and could be divided by change in transjunctional voltage to determine junctional conductance, G_j. To evaluate the transjunctional voltage dependence of the gap junctions, transjunctional voltage-clamp steps were applied between ±70 mV in 10-mV increments from a holding potential of –40 mV. The initial and steady state junctional currents were measured at 40 msec and 24 seconds, respectively, after application of the voltage-clamp step. The normalized steady state junctional conductance (G_j) versus transjunctional voltage (V_j) relation was determined by normalizing the steady state conductance values to the values at ±10 mV. The G_j–V_j relation was fit to a Boltzmann equation: G_j= G_jmin + (G_jmax -G_jmin)/{1+exp[A*(V_j -V₀)]}, where G_j is the steady state conductance, G_jmin is the minimum conductance, G_jmax is the maximum conductance, A is the cooperativity constant, and V₀ is the voltage at which the decrease in G_j is half maximal. Oocyte pairs with resting membrane potentials more negative than –15 mV were selected for analysis.

	Results

Top Abstract Introduction Materials and Methods Results Discussion References

 
Expression of Cx50D47A in Oocyte Pairs
We compared the functional properties of the D47A mutation with those of the wild-type protein by testing their ability to form gap junctional channels in the paired oocyte system. The results of these experiments are summarized in Table 1 . Oocytes injected with cRNA for D47A did not induce the formation of gap junctional channels when paired homotypically. In contrast, homotypic oocyte pairs expressing wild-type Cx50 were well coupled. Figure 1 A shows typical junctional currents from a homotypic pair expressing wild-type Cx50. The Cx50 gap junctional current rapidly inactivated to a new steady state level on application of transjunctional voltage-clamp steps to potentials greater than ±10 mV. The time course of inactivation became progressively faster at larger transjunctional potentials. Figure 1B shows a plot of the normalized steady state junctional conductance (G_j) versus transjunctional voltage (V_j) relation. G_j declined symmetrically at positive and negative V_j values. The mean G_j–V_j curve (n = 4) could be described by a Boltzmann function with G_jmax = 1.04; G_jmin = 0.16, A = 0.25 and V₀ = 22.76 mV (Table 2) . These values are similar to those previously reported by White et al.¹⁷

View larger version (11K): [in this window] [in a new window]   Figure 1. Voltage dependence of Cx50wt homotypic pairs, gap junctional current traces (A) and plot of mean normalized steady state gap junctional conductance versus transjunctional voltage (B). In (A), both cells of the pair were held at a constant holding potential and 24-second voltage-clamp steps were applied between ±70 mV in 10-mV increments. In (B), the mean normalized steady state gap junctional conductance was plotted as a function of transjunctional voltage (n = 4). The results are expressed as mean ± SEM. The solid line is the best fit of the experimental data to a Boltzmann equation with Gjmax = 1.04, Gjmin = 0.16, A = 0.25, and V0 = 22.76 mV (Table 2) .

j

To investigate further the mechanisms underlying the behavior of the D47A mutation, immunoblot analysis of membrane-enriched preparations of oocytes was performed. Oocytes injected with wild-type or mutant Cx50 cRNA synthesized a protein of approximately 70 kDa that was recognized by the anti-Cx50 monoclonal antibody 6-4-B2-C6 (Fig. 2) . The amount of wild-type and mutant Cx50 protein was similar. No major proteins were detected in antisense-injected control oocytes. These results indicate that the loss of the function without dominant inhibition exhibited by the D47A mutant was not caused by the failure of the mutant protein to reach the plasma membrane.

View larger version (33K): [in this window] [in a new window]   Figure 2. Immunoblot analysis of oocytes injected with cRNAs for mouse Cx50wt (lane 1), Cx50D47A (lane 2), and (Cx50wt+Cx50D47A) (lane 3). The plasma membrane–enriched proteins were separated on a 9% polyacrylamide gel, and then transferred to nitrocellulose. The blots were probed with the anti-Cx50 monoclonal antibody 6-4-B2-C6. All three groups of oocytes produced a 70-kDa protein band. No band was detected in antisense-treated control oocytes (data not shown).

j

j

j-

j

View larger version (31K): [in this window] [in a new window]   Figure 3. Typical junctional current traces (left) and mean Gj–Vj curves (right) for oocyte pairs injected with (A) Cx46wt, n = 3; (B) (Cx46wt+Cx50D47A), n = 4; or (C) (Cx46wt+Cx50wt), n = 1 cRNA. The experimental protocol was the same as that described in Figure 1 . The solid lines are the best fit of experimental data to a Boltzmann equation whose parameters are shown in Table 4 .

	Discussion

Top Abstract Introduction Materials and Methods Results Discussion References

The finding that the D47A mutation leads to loss of function is not surprising. The E1 loop of the connexin protein is a highly conserved and functionally important domain in gap junctional coupling and gating. The invariance of the aspartic acid at amino acid position 47 is suggestive of its importance. Mutations at this position would potentially alter the structure of the E1 loop and perturb its ability to dock with an opposing connexon.

The No2 mouse mutation has been described as semidominant because heterozygous mice have a milder form of cataract than do homozygous mice. These observations are consistent with the notion that D47A acts as a loss-of-function mutation without dominant inhibition. Consequently, cataract formation occurs when the amount of wild-type Cx50 is reduced below a critical level, and the severity of the cataract depends on the amount of reduction. In addition, the No2 mice exhibit a reduction in total ocular mass of approximately 30% compared with wild-type, suggesting that the Cx50 gap junctional channels are also involved in the regulation of growth.¹¹ A similar reduction in ocular size and diffuse nuclear opacities has been observed in homozygous Cx50 knockout mice.²¹ However, no phenotype was observed in heterozygotes suggesting that the effect of the D47A mutation cannot be completely reproduced by knocking out one allele.

Recently, a human congenital zonular pulverulent cataract has been linked to a missense mutation in human Cx50 converting proline 88 to serine.²² Unlike the D47A mutation, expression of the P88S mutant with wild-type Cx50 in Xenopus oocyte pairs results in a profound inhibition of intercellular coupling, indicating that it acts as a loss-of-function mutant with dominant inhibition.²³ It would be interesting to determine whether expression of the P88S mutation in mice by homologous recombination would result in a more severe form of cataract than does the D47A mutation.

	Acknowledgements

 
The authors thank Jay Pal for reviewing the manuscript and Xiaoqin Liu for technical assistance.

	Footnotes

 
Reprint requests: Lisa Ebihara, Department of Physiology and Biophysics, FUHS/The Chicago Medical School, 3333 Green Bay Road, North Chicago, IL 60064.

Supported by Grant EY10589 from the National Institutes of Health.

Submitted for publication December 15, 1998; accepted February 9, 1999.

Proprietary interest category: N.

	References

Top Abstract Introduction Materials and Methods Results Discussion References

 

1. Bruzzone, R, White, TW, Paul, DL (1996) Connections with connexins: the molecular basis of direct intercellular signaling Eur J Biochem 238,1-27[Medline][Order article via Infotrieve]
2. Mathias, RT, Rae, JL, Baldo, GJ (1997) Physiological properties of the normal lens Physiol Rev 77,21-50[Abstract/Free Full Text]
3. Paul, DL, Ebihara, L, Takemoto, LJ, Swenson, KI, Goodenough, DA (1991) Connexin46, a novel lens gap junction protein, induces voltage-gated currents in nonjunctional plasma membrane of Xenopus oocytes J Cell Biol 115,1077-1089[Abstract/Free Full Text]
4. White, TW, Bruzzone, R, Goodenough, DA, Paul, DL (1992) Mouse Cx50, a functional member of the connexin family of gap junction proteins, is the lens fiber protein MP70 Mol Biol Cell 3,711-720[Abstract]
5. Musil, LS, Beyer, EC, Goodenough, DA (1990) Expression of the gap junction protein connexin43 in embryonic chick lens: molecular cloning, ultrastructural localization, and post- translational phosphorylation J Membr Biol 116,163-175[Medline][Order article via Infotrieve]
6. Bergoffen, J, Scherer, SS, Wang, S, et al (1993) Connexin mutations in X-linked Charcot–Marie–Tooth disease Science 262,2039-2042[Abstract/Free Full Text]
7. Ressot, C, Gomes, D, Dautigny, A, Pham-Dinh, D, Bruzzone, R. (1998) Connexin32 mutations associated with X-linked Charcot—Marie–Tooth disease show two distinct behaviors: loss of function and altered gating properties J Neurosci 18,4063-4075[Abstract/Free Full Text]
8. Bruzzone, R, White, TW, Scherer, SS, Fischbeck, KH, Paul, DL (1994) Null mutations of connexin32 in patients with X-linked Charcot–Marie–Tooth disease Neuron 13,1253-1260[Medline][Order article via Infotrieve]
9. Kelsell, DP, Dunlop, J, Stevens, HP, et al (1997) Connexin 26 mutations in hereditary non-syndromic sensorineural deafness Nature 387,80-83[Medline][Order article via Infotrieve]
10. Britz-Cunningham, SH, Shah, MM, Zuppan, CW, Fletcher, WH (1995) Mutations of the Connexin43 gap-junction gene in patients with heart malformations and defects of laterality (see comments) N Engl J Med 332,1323-1329[Abstract/Free Full Text]
11. Steele, ECJ, Lyon, MF, Favor, J, Guillot, PV, Boyd, Y, Church, RL (1998) A mutation in the connexin 50 (Cx50) gene is a candidate for the No2 mouse cataract Curr Eye Res 17,883-889[Medline][Order article via Infotrieve]
12. Steele, EC, Jr, Lyon, MF, Glenister, PH, Guillot, PV, Church, RL (1998) Identification of a mutation in the connexin 50 (Cx50) gene of the No2 Cataractous Mouse Mutant Werner, R eds. Gap Junctions ,289-293 IOS Press Amsterdam.
13. Krieg, PA, Melton, DA (1984) Functional messenger RNAs are produced by SP6 in vitro transcription of cloned cDNAs Nucleic Acids Res 12,7057-7070[Abstract/Free Full Text]
14. Weiner, MP, Costa, GL, Schoettlin, W, Cline, J, Mathur, E, Bauer, JC (1994) Site-directed mutagenesis of double-stranded DNA by the polymerase chain reaction Gene 151,119-123[Medline][Order article via Infotrieve]
15. Ebihara, L. (1996) Xenopus connexin38 forms hemi-gap-junctional channels in the nonjunctional plasma membrane of Xenopus oocytes Biophys J 71,742-748[Abstract/Free Full Text]
16. Swenson, KI, Jordan, JR, Beyer, EC, Paul, DL (1989) Formation of gap junctions by expression of connexins in Xenopus oocyte pairs Cell 57,145-155[Medline][Order article via Infotrieve]
17. White, TW, Bruzzone, R, Wolfram, S, Paul, DL, Goodenough, DA (1994) Selective interactions among the multiple connexin proteins expressed in the vertebrate lens: the second extracellular domain is a determinant of compatibility between connexins J Cell Biol 125,879-892[Abstract/Free Full Text]
18. Kistler, J, Kirkland, B, Bullivant, S. (1985) Identification of a 70,000-D protein in lens membrane junctional domains J Cell Biol 101,28-35[Abstract/Free Full Text]
19. Jiang, JX, Goodenough, DA (1996) Heteromeric connexons in lens gap junction channels Proc Natl Acad Sci USA 93,1287-1291[Abstract/Free Full Text]
20. Zampighi, GA, Simon, SA, Hall, JE. (1992) The specialized junctions of the lens Int Rev Cytol 136,185-225[Medline][Order article via Infotrieve]
21. White, TW, Goodenough, DA, Paul, DL (1998) Targeted ablation of connexin50 in mice results in microphthalmia and zonular pulverulent cataracts J Cell Biol 143,815-825[Abstract/Free Full Text]
22. Shiels, A, Mackay, D, Ionides, A, Berry, V, Moore, A, Bhattacharya, S. (1998) A missense mutation in the human connexin50 gene (GJA8) underlies autosomal dominant "zonular pulverulent" cataract, on chromosome 1q Am J Hum Genet 62,526-532[Medline][Order article via Infotrieve]
23. Pal JD, Mackay D, Shiels A, Berthoud VM, Beyer EC, and Ebihara L. Molecular mechanisms underlying a missense mutation in human connexin 50 associated with congenital cataracts. American Journal of Physiology, June 1999 (in press).

This Article Abstract Full Text (PDF) Submit a response Alert me when this article is cited Alert me when eLetters are posted Alert me if a correction is posted Citation Map Services Email this article to a friend Similar articles in this journal Similar articles in PubMed Alert me to new issues of the journal Download to citation manager Citing Articles Citing Articles via Google Scholar Google Scholar Articles by Xu, X. Articles by Ebihara, L. Search for Related Content PubMed PubMed Citation Articles by Xu, X. Articles by Ebihara, L.