Article |
Address correspondence to Thomas W. White, Dept. of Physiology and Biophysics, BST 5-147, State University of New York, Stony Brook, NY 11794-8661. Tel.: (631) 444-9683. Fax: (631) 444-3432. E-mail: thomas.white{at}sunysb.edu
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Abstract |
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Key Words: knockin; knockover; connexin; lens; intercellular communication
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Introduction |
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There are at least 20 connexin genes in vertebrates, and most organs express a distinct subset of these, suggesting that biochemical coupling may be finely tuned to meet the needs of each tissue (Bruzzone et al., 1996; Willecke et al., 2002). This hypothesis was confirmed by studies of genetically manipulated mice that showed a restricted ability of connexins to substitute for one another in vivo (Plum et al., 2000; White, 2002). An excellent example of this lack of redundancy is provided by the lens, which predominantly expresses two connexins, Cx46 and Cx50. In mice, knockout of Cx50 resulted in significantly reduced lens growth and mild nuclear cataracts (White et al., 1998; Rong et al., 2002). In contrast, deletion of Cx46 produced severe cataracts without altering ocular growth (Gong et al., 1997). Homozygous replacement of the Cx50 coding region with that of Cx46 by genetic knockin corrected the nuclear cataracts but not the growth deficit that resulted from knockout of the Cx50 gene (White, 2002). Together, these studies suggested that a loss of connexin diversity prevented normal lens development and that distinct modes of coupling provided by Cx46 and Cx50 were required.
The lens is composed of only two distinct types of cell, a simple epithelium lining the anterior surface and highly differentiated fibers that constitute the rest of the lenticular mass (White and Bruzzone, 2000b). Epithelial cells undergo mitosis and differentiate to give rise to new lens fibers, which lose intracellular organelles and accumulate high concentrations of crystallins to produce the high refractive index needed for accommodation. Gap junctional communication joins all the cells of the lens into a functional syncytium (Miller and Goodenough, 1986; Rae et al., 1996), and this feature allows the metabolically active epithelium to maintain in fiber cells the precise intracellular conditions necessary to prevent precipitation of the crystallins and cataract formation (Mathias et al., 1997). These processes of epithelial cell division and fiber differentiation continue throughout life at the lens equator, adding new fibers to the lens surface that enshroud older fibers and produce radially symmetric lens growth.
In the mouse lens, Cx50 and Cx46 have distinct but overlapping patterns of gene expression. Cx50 is abundantly transcribed in epithelial cells and continues to be expressed in the differentiating lens fibers (Rong et al., 2002). In contrast, Cx46 is poorly represented in the lens epithelium but undergoes a large up-regulation coincident with fiber differentiation (Gong et al., 1997). It follows that animals heterozygous for the knockin gene would coexpress these two connexins in a novel subset of cells where they could potentially mix together into the same intercellular channels (White and Bruzzone, 1996, 2000a; Beyer et al., 2001). Mixing of connexin subunits in such heteromeric channels would continue to provide ionic communication (Brink et al., 1997) but could dramatically alter the range of biochemical solutes shared between coupled cells (Bevans et al., 1998; Beyer et al., 2001). Cx46 and Cx50 can mix together to form heteromeric channels in vivo, and these channels provide a robust ionic coupling in vitro (Jiang and Goodenough, 1996; Hopperstad et al., 2000).
Here we have used mouse genetics to manipulate the connexin content of the Cx46 and Cx50 loci at will. We show that forced mixing of Cx46 and Cx50 in heterozygous knockin mice did little to diminish ionic coupling, or the biochemical coupling required for normal growth, but dominantly interfered with the biochemical coupling required for lens clarity. We also show that Cx46, when expressed alone from the Cx50 locus in knockover animals, could maintain lens clarity without supporting normal growth. These results imply that lens intercellular communication is highly specialized and that normal growth and differentiation are not regulated by the magnitude of ionic coupling. More precisely, the data suggest distinct modes of biochemical coupling provided by Cx46 and Cx50 are required for homeostasis. In addition, the results obtained with these mice offer a novel mechanistic insight into the pathology of human cataracts that result from dominant mutations in lens connexin genes (Francis et al., 1999; White and Paul, 1999; Graw and Loster, 2003).
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Results |
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Heterozygous knockin lenses grow normally
The interbreeding of genetically engineered animals also allowed dissection of the potentially overlapping influences of Cx50 quantity and mixing on lens growth. Knockout of Cx50 impaired lens growth in addition to causing cataract (White et al., 1998; Rong et al., 2002), and the impaired growth phenotype was not rescued by homozygous knockin of Cx46 (White, 2002). In both cases, the impaired growth rate was most evident in early postnatal life. To determine if heterozygous knockin lenses grew normally, lens mass was quantified as a function of age. As shown in Fig. 3 A, there were no significant differences in the growth rate of wild-type and heterozygous knockin [Cx46(+/+) Cx50(+/46)] lenses between 2 and 12 wk of age, a period in which the Cx50-deficient lenses clearly manifest a growth defect (White et al., 1998; White, 2002).
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Histology of heterozygous knockin lenses
Cataractogenesis in the Cx46 and Cx50 knockout lenses initiated in the early postnatal period (Gong et al., 1997; White et al., 1998). To examine this developmental stage of heterozygous knockin lenses for pathological changes, juvenile eyes were fixed, serially sectioned, and stained with hematoxylin and eosin. Examination of the equatorial regions of lenses of all genotypes at low magnification (Fig. 4, AC) showed normal cell elongation, accumulation of high concentrations of eosinophilic cytoplasmic protein, and loss of fiber cell nuclei with age, all markers of normal fiber differentiation (Wride, 1996). However, prominent differences in lens histology were detected in the more centrally located fiber cells that are highly dependent on junctional communication for nutrient exchange.
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Cataracts contain precipitated crystallins
During normal differentiation, lens fibers express a highly specialized group of cytoplasmic proteins called crystallins (Wride, 1996). A characteristic feature of many lens opacities is the conversion of soluble crystallins into an insoluble form (Piatigorsky, 1980), which was observed in both the Cx46 and Cx50 knockout mice (Gong et al., 1997; White et al., 1998) and corrected in homozygous knockin animals (White, 2002). Therefore, the effect of knockin heterozygosity on the solubility of crystallin proteins was examined. Wild-type and heterozygous knockin [Cx46(+/+) Cx50(+/46)] lenses from adult animals were separated into soluble and insoluble components that were analyzed by Western blotting for A-,
B-, ß-, and
-crystallins. All four of the crystallin proteins examined were highly abundant in the soluble fractions from either genotype of lens (Fig. 5, lanes 1 and 2), demonstrating that the changes in gene transcription and translation that accompany fiber differentiation occurred normally in the heterozygous knockin animals.
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Heterozygous lenses are well coupled ionically
The inappropriate mixing of Cx46 and Cx50 in heterozygous knockin mice perturbed normal crystallin solubility and produced cataracts, an outcome which did not occur in wild-type or homozygous knockin lenses (White, 2002). This defect could have resulted from a perturbation of normal patterns of either ionic or biochemical coupling, or a reduction in the magnitude of both. To determine the extent of gap junctional communication in heterozygous knockin lenses [Cx46(+/+) Cx50(+/46)], we directly quantified the intercellular passage of ions using electrical impedance techniques (Mathias et al., 1981). Young adult lenses (46 wk old) were impaled at a 45° angle from the anterior posterior axis, and the electrical series resistance (Rs) was recorded at different radial depths. In both wild-type and heterozygous knockin lenses, Rs increased at greater depths consistent with the increasing number of fiber cells coupled by low resistance gap junctions between the recording electrode and the lens surface (Fig. 6 A). Conversion of these Rs data to values of resistivity allowed for averaging the initial 20% of lens fiber depth and showed an 24% increase in resistivity in heterozygous knockin animals (Fig. 6 B). This slight increase in resistance was consistent with the fact that the unitary conductance of Cx46 is smaller than Cx50, and functional replacement of one copy of Cx50 with one copy of Cx46 should result in a net reduction of ionic coupling if the total number of open channels remained constant.
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Heterozygous lenses exhibit restricted dye coupling
Documenting the actual intercellular metabolites responsible for the observed cataractogenesis is technically challenging (Goldberg et al., 1999, 2002), but fluorescent dyes can be qualitatively used to reveal approximate patterns of biochemical coupling within the living lens (Miller and Goodenough, 1986; Rae et al., 1996; White et al., 1998). Our data suggest that heterozygous knockin lenses uniquely coexpress Cx46 and Cx50 in the lens epithelium, and this may have altered biochemical coupling within these cells. To determine if the extent of epithelial dye coupling was altered, we directly visualized the intercellular passage of DAPI. This dye was chosen for two reasons; first DAPI accumulates and concentrates within the nuclei of cells, and second, its intercellular passage has been shown to be highly dependent on which connexin isoforms are providing intercellular coupling (Elfgang et al., 1995; Cao et al., 1998). Since the only nuclei in the central anterior surface of the lens are within the underlying monolayer of epithelial cells (Fig. 4), these two features made DAPI an ideal candidate to probe qualitative changes in biochemical coupling in the intact lens epithelium.
Young adult lenses (46 wk old) were impaled through the central anterior capsule, and the resting membrane voltage was monitored throughout the injection. In four out of four trials, injection of a single epithelial cell in wild-type lenses [Cx46(+/+) Cx50(+/+)] resulted in the intercellular passage of DAPI to a large number of neighboring cells (Fig. 7 A). The dye spread pattern in wild-type lenses tended to be more extensive along the axis of the underlying fiber cells, which radiate outward from the anterior suture and are highly coupled to the epithelium (Rae et al., 1996; White et al., 1998). In contrast, DAPI was transferred to many fewer neighboring epithelial cells (≤10) in heterozygous knockin lenses [Cx46(+/+) Cx50(+/46)] in five independent injections (Fig. 7 B). Thus, DAPI was able to pass through gap junctions in all lenses, but there was also a large qualitative difference in the extent of dye spread. Proper quantitation of dye permeation and selectivity is highly laborious (Valiunas et al., 2002) and well beyond the scope of the present study, but these qualitative differences between wild-type and heterozygous knockin lenses support our hypothesis that biochemical coupling was altered by the forced coexpression of Cx46 and Cx50 in epithelial cells.
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Discussion |
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As a solid avascular sphere, the lens is an organ that is uniquely dependent on gap junctional communication for providing nutrients and removing metabolic wastes (Piatigorsky, 1980; Mathias et al., 1981). A microcirculation model that relies on ionic coupling through gap junctions generates the osmotic fluxes and voltage gradients that drive biochemical modes of coupling in the lens (Donaldson et al., 2001). Briefly, an ionic current enters the lens along the extracellular spaces between cells. After crossing fiber cell membranes in the lens interior, the current flows back toward the surface via an intracellular pathway provided by ionic coupling through gap junction channels. The circulating current generates fluid flow and a voltage gradient, forces which in turn help carry larger biochemical solutes into the lens and between the coupled cells (Mathias et al., 1997). In Cx46 knockout mice, this ionic current was completely lost in the inner lens fibers resulting in severe cataracts (Gong et al., 1997, 1998). In the Cx50 knockout, the inner ionic current was reduced 66% compared with wild-type, producing a milder cataract phenotype (White et al., 1998; Baldo et al., 2001). In support of our conclusion that altered biochemical coupling alone can produce cataract, heterozygous knockin lenses [Cx46(+/+) Cx50(+/46)] retained high levels of ionic coupling, which presumably reflected a normally operating microcirculation, yet they displayed a severe cataract.
Surprisingly, knockover lenses [Cx46(-/-) Cx50(46/46)] lacked the cataract normally resulting from either Cx46 or Cx50 knockout (Gong et al., 1997; White et al., 1998). In the Cx46 knockout, Cx50 expression from its native locus was unable to maintain clarity, whereas Cx46 expression from the Cx50 locus in the knockover prevented cataract. As many prior studies have established that levels of Cx46 and Cx50 protein synthesis show no apparent compensatory up-regulation after genetic manipulation (Gong et al., 1998; White et al., 1998, 2001; Baldo et al., 2001; Rong et al., 2002; White, 2002), Cx46 would be expected to provide a lower level of ionic coupling than Cx50 when expressed from the same promoter, due to its smaller unitary conductance (140 pS versus 220 pS). At the very least, knockover lenses would be expected to have less ionic coupling than wild-type due to an overall reduction in channel number. These data suggest that the combination of ionic and biochemical coupling provided by Cx46, when exclusively expressed from the Cx50 locus, was far more efficient than that provided by Cx50 in maintaining lens clarity.
Lens growth results from the regulated proliferation of epithelial cells that migrate toward the equatorial region where they differentiate into new fiber cells (Wride, 1996). Since homozygous knockin of Cx46 failed to rescue growth (White, 2002), it was not surprising that the knockover lenses displayed the same lens growth defect as the Cx50 knockout. It was less obvious why heterozygous knockin lenses were able to grow normally despite having severe cataracts. The fact that this normal growth was evident regardless of whether the native Cx46 gene was even present suggests that lens growth, like clarity, was not dependent on the overall magnitude of coupling and that the incongruous mixing of Cx46 and Cx50 did not alter the biochemical coupling that participates in the regulation of epithelial proliferation and fiber differentiation. Normal lens growth was also observed in heterozygous Cx50 knockouts (White et al., 1998; Rong et al., 2002), implying that one allele of Cx50 provides sufficient biochemical coupling. Consistent with this, we have seen that lenses lacking both alleles of Cx46 and one copy of Cx50 [Cx46(-/-) Cx50(+/-)] still grow normally (unpublished data). Together, these data suggest that normal lens growth only requires one copy of Cx50 and is independent of the remaining connexin composition of the lens.
In wild-type mice, Cx46 and Cx50 are normally coexpressed in fibers but not in the lens epithelium. Additionally, they are known to naturally cooligomerize into heteromeric channels within the fiber cells (Konig and Zampighi, 1995; Jiang and Goodenough, 1996), and heteromeric channels composed of Cx46 and Cx50 provide robust levels of ionic conductance in vitro (Ebihara et al., 1999; Hopperstad et al., 2000). In the knockin mice, our immunocytochemistry data showed that Cx46 was translocated into the epithelium where it could inappropriately mix with Cx50 in heterozygous animals. Heteromeric mixing of connexins has been documented to profoundly alter the biochemical coupling of signaling molecules such as cyclic nucleotides or fluorescent dyes that mimic their size and charge (Bevans et al., 1998; Valiunas et al., 2002). This novel mixing of Cx46 and Cx50 in lens epithelial cells produced a dominant cataract phenotype that was much more severe than the Cx50 knockout phenotype and was also independent of total lens connexin stoichiometry or quantity. From the data presented here, we conclude that incongruous mixing of Cx46 and Cx50 in epithelial cells altered the spatial patterns of biochemical coupling necessary to sustain lens clarity.
Ideally, one would like to directly document the proposed changes in biochemical coupling in the lens responsible for the observed cataractogenesis, but this is technically difficult, especially in a three-dimensional optically active tissue. Instead, we have shown that DAPI permeation was qualitatively different in the epithelial cells of heterozygous knockin lenses compared with wild-type lenses. DAPI has a similar charge and molecular mass as many cytoplasmic signaling molecules, and it is not unreasonable to assume that alterations in this dye's spread may reflect changes in permeation in other types of endogenous metabolites. In any case, we have also shown by impedance techniques that intercellular communication to ions was not disrupted in the heterozygous knockin lenses and that our impedance data were quantitatively reconciled with an approximately one to one replacement of functional channels if one considered differences in the unitary conductance of Cx46 and Cx50 (Srinivas et al., 1999; Hopperstad et al., 2000). If one accepts that the principal mechanism used by connexin channels to convey information between cells is intercellular coupling to ions and small metabolites, then our data showing high levels of ionic coupling and altered dye spread logically infer that altered biochemical coupling must be responsible for cataracts in the heterozygous knockin mice.
This explanation also provides a potential mechanistic insight into the pathology of human congenital cataracts caused by mutations in connexin genes (Francis et al., 1999; White and Paul, 1999; Graw and Loster, 2003). To date, only dominant cataracts caused by heterozygous missense mutations in Cx50 have been identified, and these patients generally exhibit normal eye and lens growth (Shiels et al., 1998; Francis et al., 1999; Polyakov et al., 2001). In contrast, the recessive phenotype of the Cx50 knockout mice includes microphthalmia in addition to cataracts (White et al., 1998; Rong et al., 2002). The heterozygous knockin lenses [Cx46(+/+) Cx50(+/46)] described in this article offer a resolution to this discrepancy, since the knockin allele behaves like a dominant mutation. Like the human cataract pedigrees, one normal Cx50 allele is sufficient to ensure normal lens growth, and one altered Cx50 allele is sufficient to disrupt homeostasis and cause cataract. It is highly improbable that all of the missense connexin mutants associated with cataracts will be devoid of functional activity, since a subset of missense mutations associated with other connexin disorders have been shown to retain gap junction channel activity in vitro (Oh et al., 1997; Ressot et al., 1998; Bruzzone et al., 2003). Our results expand the pathological paradigm and now allow for the consideration of functional mutant, or incongruously expressed wild-type, connexins to dominantly alter biochemical communication without disrupting ionic coupling.
A summary of our current and previously published data (Table I) shows an emerging pattern of connexin-specific gap junction functions in the lens. The two predominant connexins of the lens fulfill unique functions; Cx46 is primarily responsible for maintaining lens clarity, whereas Cx50 mainly provides for normally regulated growth. In addition, the contributions of Cx50 to normal growth and the maintenance of clarity are independent of each other, and Cx46 better fulfills the latter role in the knockover animals [Cx46(-/-) Cx50(46/46)]. Here, we have shown that connexin-specific differences in biochemical coupling differentially regulate lens growth and clarity and that the spectrum of larger biochemical solutes that need to be exchanged between lens cells is indeed finely tuned to meet the needs of this tissue.
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Materials and methods |
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Growth analysis
Lenses from eyes of age-matched animals were dissected, blotted dry on tissue paper, and individually weighed. Differences between lenses from various genotypes were compared by the Student's unpaired t test.
Microscopy
Eyes were dissected and immediately transferred to Petri dishes containing prewarmed M199 medium with Hanks Salts (M199) on a 37°C stage. Lenses were dissected and transferred to prewarmed poly-lysinecoated Petri dishes with glass bottoms (World Precision Instruments) filled with M199. Lenses were oriented onto their equatorial edges and photographed on an Olympus SZX9 microscope equipped with an Olympus C3030 zoom digital camera.
Immunofluorescence
Adult eyes were dissected, cut open at the posterior pole, fixed in 1% formaldehyde in PBS overnight, rinsed in PBS, and embedded in Optimal Cutting Temperature compound in liquid N2. Frozen sections (1012 µM) were cut on a cryostat, air dried onto Superfrost Plus slides, and blocked with 3% BSA in PBS. Sections were stained with rabbit antisera against Cx46 (Paul et al., 1991), diluted in 3% BSA in PBS, and washed with PBS. Primary antisera were visualized with a Cy3-conjugated goat antirabbit antibody (Jackson ImmunoResearch Laboratories) and photographed on an Olympus BX51 microscope using an Optronics MagnaFire digital camera.
Histology
Postnatal day 7 eyes were dissected, cut open at the posterior pole, fixed in 4% formaldehyde in PBS overnight, rinsed in PBS, and dehydrated through an ethanol series. Eyes were cleared in xylene and embedded in paraffin. Paraffin sections (23 µM) were cut on a 0.5-cm diamond knife, floated on water, and dried onto Superfrost Plus slides overnight at 37°C. Sections were stained with hematoxylin and eosin and photographed.
Western blotting
Lenses were dissected, and equal wet weights were homogenized in 0.1 M NaCl, 0.1 M Na2HPO4, 10 mM ascorbic acid, and protease inhibitors (10 µg/ml each of chymostatin, leupeptin, and pepstatin). After centrifugation at 14,000 g for 20 min at room temperature, the soluble fraction was recovered and stored at -80°C. The insoluble fraction was subjected to a second wash with 1 ml of 0.1 M NaCl, 0.1 M Na2HPO4 followed by a subsequent wash with 1 ml of 20 mM NaOH. The insoluble fraction was finally washed in 1 ml of 1 mM Na2CO3 after which the pellets were resuspended in sample buffer and stored at -80°C. Equal aliquots of samples from each genotype were electrophoresed on 10% SDSpolyacrylamide gels, transferred to nitrocellulose membranes, and incubated with antibodies specific for A-,
B-, ß-, and
-crystallin proteins. Primary antibodies were detected with alkaline phosphataseconjugated goat antirabbit IgG (Jackson ImmunoResearch Laboratories) using nitro blue tetrazolium and 5-bromo-4-chloro-3-indolyl phosphate as substrates (Sigma-Aldrich).
Impedance
Gap junctional ionic coupling was measured as described previously (Gong et al., 1998; Baldo et al., 2001). Briefly, lenses were dissected and placed anterior surface down into a 37°C chamber filled with Tyrode solution (138 mM NaCl, 5.4 mM KCl, 1 mM MgCl2, 10 mM glucose, 5 mM Hepes, pH 7.4). A stochastic current containing a wide range of frequencies was passed through a microelectrode into a fiber cell near the center of the lens, while the induced voltage was recorded with a second electrode placed at different radial depths from the lens surface. Voltage and current data were input into a fast Fourier analyzer to compute the real time frequency domain impedance. Gap junctional ionic coupling was calculated from impedance data using previously described models (Mathias et al., 1981; Baldo et al., 2001).
Dye coupling
Gap junctional coupling to dyes mimicking larger biochemical solutes was measured as described previously (White et al., 1998). Briefly, 46-wk-old lenses were dissected and mounted on their posterior surface on poly-L-lysinecoated 35-mm Petri dishes filled with 37°C M199. High resistance microelectrodes were filled with 1 mg/ml DAPI (Molecular Probes) dissolved in 120 mM K-aspartate, 10 mM NaCl, 1 mM MgCl2, 3 mM Mg-ATP, and 5 mM Hepes, pH 7.2. Centrally located epithelial cells were impaled through the lens capsule from the anterior lens surface. DAPI was iontophoretically injected for 5 min, while continuously monitoring the membrane potential of the impaled cell. Injected lenses were photographed on an Olympus BX51 microscope using an Optronics MagnaFire digital camera.
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Acknowledgments |
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Submitted: 11 March 2003
Revised: 24 April 2003
Accepted: 24 April 2003
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References |
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