May 2009
Volume 50, Issue 5
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Retina  |   May 2009
Defining the Residual Vision in Leber Congenital Amaurosis Caused by RPE65 Mutations
Author Affiliations
  • Samuel G. Jacobson
    From the Department of Ophthalmology, Scheie Eye Institute, University of Pennsylvania, Philadelphia, Pennsylvania; the
  • Tomas S. Aleman
    From the Department of Ophthalmology, Scheie Eye Institute, University of Pennsylvania, Philadelphia, Pennsylvania; the
  • Artur V. Cideciyan
    From the Department of Ophthalmology, Scheie Eye Institute, University of Pennsylvania, Philadelphia, Pennsylvania; the
  • Alejandro J. Roman
    From the Department of Ophthalmology, Scheie Eye Institute, University of Pennsylvania, Philadelphia, Pennsylvania; the
  • Alexander Sumaroka
    From the Department of Ophthalmology, Scheie Eye Institute, University of Pennsylvania, Philadelphia, Pennsylvania; the
  • Elizabeth A. M. Windsor
    From the Department of Ophthalmology, Scheie Eye Institute, University of Pennsylvania, Philadelphia, Pennsylvania; the
  • Sharon B. Schwartz
    From the Department of Ophthalmology, Scheie Eye Institute, University of Pennsylvania, Philadelphia, Pennsylvania; the
  • Elise Heon
    Department of Ophthalmology and Vision Sciences, The Hospital for Sick Children, University of Toronto, Toronto, Ontario, Canada; and the
  • Edwin M. Stone
    Howard Hughes Medical Institute and Department of Ophthalmology, University of Iowa Hospitals and Clinics, Iowa City, Iowa.
Investigative Ophthalmology & Visual Science May 2009, Vol.50, 2368-2375. doi:10.1167/iovs.08-2696
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      Samuel G. Jacobson, Tomas S. Aleman, Artur V. Cideciyan, Alejandro J. Roman, Alexander Sumaroka, Elizabeth A. M. Windsor, Sharon B. Schwartz, Elise Heon, Edwin M. Stone; Defining the Residual Vision in Leber Congenital Amaurosis Caused by RPE65 Mutations. Invest. Ophthalmol. Vis. Sci. 2009;50(5):2368-2375. doi: 10.1167/iovs.08-2696.

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      © ARVO (1962-2015); The Authors (2016-present)

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Abstract

purpose. To quantify the residual vision in Leber congenital amaurosis (LCA) caused by RPE65 mutations.

methods. Patients with RPE65-LCA (n = 30; ages, 4–55) were studied using electroretinography (ERG), full-field stimulus testing (FST), kinetic and static threshold perimetry, and optical coherence tomography (OCT).

results. All patients with RPE65-LCA had abnormal ERGs even at the youngest ages. There were no detectable rod ERGs and only reduced cone ERGs. By chromatic FST, however, 59% of patients had measurable rod- and cone-mediated function. The remaining 41% had only cone-mediated function. Extent of kinetic fields varied widely in the first two decades of life but, by the end of the third decade, there was very little measurable field. Regional patterns of visual loss were evident using dark-adapted static threshold perimetry. The mildest dysfunctions showed relatively homogeneous sensitivity loss beyond the central field. Mid-peripheral dysfunction was a later feature; finally, only central and peripheral islands remained. Colocalized measures of visual function and retinal structure by OCT showed that visual function was detectable when a photoreceptor layer was detectable.

conclusions. Residual rod as well as cone function is detectable in RPE65-LCA. The finding of different regional patterns of visual loss in these patients suggests that the optimal retinal site(s) for subretinal gene delivery to achieve efficacy are likely to change with disease progression.

Leber congenital amaurosis (LCA) is a molecularly heterogeneous group of autosomal recessive diseases with early onset of severe visual loss. 1 One molecular form of LCA is due to mutations in the gene encoding RPE65 (retinal pigment epithelium-specific 65 kDa protein). Scientific interest in RPE65 is high because this molecule is the long-sought isomerohydrolase of the visual cycle. 2 3 4 Medical interest has also been piqued by proof-of-concept experiments showing restored vision in two species of Rpe65-deficient animals by subretinal gene replacement therapy 5 6 7 8 9 10 and now in human clinical trials. 11 12 13 14  
Despite this remarkable progress, human RPE65-LCA disease remains incompletely understood. We know that severely impaired vision is associated with inheritance of two RPE65 alleles which show little or no isomerohydrolase activity in vitro. 15 A visual toll is taken on both central and peripheral vision and on both rod and cone photoreceptor-mediated function (reviewed in Ref. 16 ). Unlike Rpe65-deficient animal models at early ages and stages, children with early visual dysfunction also have a serious retinal degeneration. 9 17 18 The retinal degeneration component tends to be masked by dysfunction resulting from the visual cycle abnormality, but eventually there is clinically apparent pigmentary retinopathy and chorioretinal atrophy. 16 Adding to the complexity is the fact that the visual cycle blockade in humans and animals is obviously not complete, because there is residual vision. Animal models with Rpe65 deficiency have residual photoreceptor function. 5 6 19 20 21 In mutant mice, the residual function has been ascribed to either low levels of production of 11-cis-retinal or Rpe65-independent pathways. 21 22  
The goal of the present study was to determine quantitatively key features of the residual vision in a population of patients with RPE65-LCA. We inquired whether the residual function was only cone- or also rod-mediated by using electroretinography (ERG) and full-field sensitivity testing (FST). The pattern of visual loss across the retina was explored with kinetic and dark-adapted static perimetry. The results have implications, not only for understanding the human disease but also for enhancing strategies for therapy of RPE65-LCA. 
Materials and Methods
Subjects
There were 30 patients (age range, 4–55) with RPE65 mutations, representing 26 families (Table 1) . Also included were data from an 8-year-old patient with autosomal dominant retinitis pigmentosa (adRP) caused by a rhodopsin (RHO) gene mutation. Normal subjects (n = 16; age range, 20–61) were also included. All patients with RPE65-LCA had a history of poor vision and nystagmus from infancy. A complete ophthalmic examination and visual function studies were performed (Table 1) . Informed consent and assent were obtained; procedures adhered to the guidelines in the Declaration of Helsinki and were approved by the institutional review board. 
Psychophysical Testing
Full-field stimulus testing (FST) was performed as previously described. 25 26 In brief, dark-adapted sensitivity to a full-field stimulus was measured in patients with RPE65-LCA (n = 22; age range, 5–46) using white, red, or blue flashes (200-ms duration) delivered with an LED-based, computer-driven stimulator (Colordome; Diagnosys LLC, Littleton, MA), and followed published procedures. 26 The white stimulus was used to quantify the level of sensitivity. FST loss was defined as the difference between mean normal and patient FST sensitivity. The sensitivity difference (blue-red) to chromatic stimulation was used to evaluate whether rods, cones, or both photoreceptor systems mediate perception. Cone-mediated perception is expected to yield nearly equal sensitivity values (blue-red difference, <3.1 dB) for both colors. Rod-mediated perception would yield a blue-red difference >19.3 dB. Values between those limits indicate that rods are mediating blue detection and cones are mediating red (mixed mediation). 25 Small differences in sensitivity peaks between rhodopsin and isorhodopsin 22 are not expected to be discernible by the FST method. 
Kinetic perimetry was performed with targets V-4e and I-4e; the V-4e results were quantified with published methods. 27 Dark-adapted static threshold perimetry was performed with a modified automated perimeter (Humphrey Field Analyzer; Carl Zeiss Meditec Inc, Dublin, CA) and achromatic (white) stimuli (1.7° diameter; 200-ms duration) presented in a 12° grid across the visual field (71 extrafoveal locations). 28 It is important to note that the maximum intensity of the white stimulus from this automated perimeter is 1 log unit higher than that of the kinetic perimeter. An average of additional measurements performed at fixation and in a 4° grid centered at fixation was used as a sensitivity estimate for the most central location, which is plotted as a single value at 0° eccentricity. Psychophysical thresholds were also measured at 2° intervals spanning 60° along the horizontal and vertical meridians crossing fixation. Techniques, methods of data analysis and normal results have been described. 25 27 28 In a subset of patients (n = 13) and normal subjects (n = 4), dark-adapted sensitivity was plotted as a function of eccentricity in each subject. For central locations (within 10°) the data were obtained from horizontal sensitivity profiles with greater spatial resolution (see above). Sensitivity values at equal eccentricities were averaged. 
Electroretinography
Full-field electroretinograms (ERGs) were performed in 29 patients with a standard protocol. Details of the methods and normal results have been published. 27 29 Reproducibility of small-amplitude flicker waveforms was validated by comparing several independent recordings. 30 In four patients, high-energy stimuli from a custom-built xenon flash stimulator (luminance of unattenuated white flash, 3.4 log cd · s · m−2; duration: ∼1 ms) were used to attempt to record ERG photoresponses under dark-adapted conditions. Details of the methodology and normal results have been published. 31 32  
Optical Coherence Tomography (OCT)
Cross-sectional retinal reflectivity profiles were obtained with OCT in 20 patients by using one of two instruments (OCT3 [Humphrey Instruments; Carl Zeiss Meditec, Inc.], with a resolution of ∼8 μm (n = 6 patients), and the RTVue-100 (n = 14) [Optovue Inc., Fremont, CA], with a 5-μm axial resolution in tissue). Details of our recording and analysis techniques have been published. 18 23 33 34 Retinal cross sections were sampled with vertical scan groups centered on the anatomic fovea and consisting of five overlapping segments of linear scans, each 4.5 mm in length, extending 9 mm in either direction. Each segment was repeated at least three times. A video fundus image showing the location of the scanned segment was acquired and saved with each OCT scan by the commercial software. Post-acquisition processing of OCT data was performed with custom programs written in commercial software (MatLab 6.5; MathWorks, Natick, MA). Longitudinal reflectivity profiles (LRPs) making up the OCT scans were aligned by using a dynamic cross-correlation algorithm. 33 A manual override was used when crossing structures which interrupted local lateral isotropy by shadowing deeper signals. Nuclear layers were defined as previously published. 9 33 34 The outer photoreceptor nuclear layer (ONL) thickness was defined as the major intraretinal signal trough delimited by the signal slope maxima. ONL thickness was related to colocalized psychophysical thresholds determined by dark-adapted static perimetry along the same retinal regions. ONL thickness values were laterally averaged at 0.6-mm intervals to correspond with the lateral sampling of vision. For analysis pairs of colocalized measures of ONL thickness-sensitivity data from all patients were binned at 10-μm thickness intervals. ONL thickness values ≤5 μm were considered not detectable (ND). 
Results
Residual Function in RPE65 Deficiency: Cones, Rods, or Both
ERGs were abnormal in all patients with RPE65-LCA tested. There were no detectable waveforms in 41% of the patients tested, and the other 59% had signals to only some stimuli (described later). Representative ERGs in RPE65-LCA were compared with normal waveforms and those from a disease with primary rod dysfunction, autosomal dominant retinitis pigmentosa (adRP) caused by rhodopsin (RHO) gene mutation (Fig. 1A) . The normal ERG to a dim blue light flash in the dark-adapted state represents a rod-mediated b-wave. A white light flash, dark-adapted, elicits a faster and larger waveform with both rod and cone (i.e., mixed) contributions, but is rod dominated. Cone ERGs are recordable in the light-adapted state to single flashes of light or to flickering light at 29 Hz. Severe early-onset rod disease and residual (but abnormal) cone function is exemplified by an 8-year-old patient with adRP who had the R135L RHO mutation. There was no measurable rod b-wave and, unlike the normal, waveforms elicited with white light stimuli in the dark- and light-adapted states were similar in shape and magnitude. There was a retained but abnormal flicker signal. 
None of the patients with RPE65-LCA showed ERG responses to the dim blue light stimuli that normally evoke rod b-waves (Fig. 1A) . Twelve patients (P1, P2, P13, P16, P19, P22, P23, P25–P28, and P30) had no detectable ERGs to any stimuli; eight patients (P5, P7, P8, P11, P15, P18, P21, and P24) had only small amplitude (range, 2–4 μV) flicker ERGs; and nine patients (P3, P4, P6, P9, P10, P12, P14, P17, and P20) showed similar responses to dark- and light-adapted white stimuli and flicker waveforms with amplitudes ranging from 4 to 35 μV (normal mean ± SD = 172 ± 35 μV). We also used bright flashes to elicit ERGs in four patients (P5, P17, P18, and P22); there were no detectable responses (data not shown). In summary, the detectable ERGs in RPE65-LCA showed the pattern of a retinopathy with such severe rod dysfunction that it is not detectable with this technique; residual and abnormal cone function were measurable in many of the patients. 
FST was performed in 22 patients with RPE65-LCA by using white and chromatic stimuli (Fig. 1B) . Sensitivity to the white stimulus in the patients with RPE65-LCA was abnormally reduced and showed a range of results representing sensitivity losses of 34 to 69 dB (Fig. 1B , left). Chromatic measurements showed that more than half of the patients (13/22; 59%; age range, 6–27 years; mean age, 16) had rod mediation of the blue stimulus, indicating that there was severely reduced but detectable residual rod function. The remaining patients (9/22; 41%; age range, 5–46 years; mean age, 24) detected both red and blue stimuli with cone-mediated vision (Fig. 1B , right). It can be concluded that residual rod function (and not only cone function) is detectable by psychophysics in patients with RPE65-LCA. There was no clear relationship of patient age to presence of residual rod function. 
Localization of Residual Vision in the Visual Field
Kinetic visual fields with V-4e, a large bright target, were measurable in 29 of 30 patients. None of the patients was able to detect I-4e, the small bright target. A normal extent of kinetic field (defined as ≥90% for V-4e 27 ) was present in four patients (P8, P12, P14, and P20) at ages 10, 12, 19, and 23, respectively; there were no absolute scotomas detectable within these fields. The kinetic field of P20 at age 23 (Fig. 2A , top left) exemplifies this pattern. Other patients (n = 13; age range, 4–33 years) showed sizeable fields that were generally constricted and had reduced extent (39%–88% of normal). Such patterns are exemplified by P3 at age 6 (Fig. 2A , top center). Later stage patterns showed either a residual central island, with or without peripheral islands, or only a far peripheral island (Fig. 2A , right: P24, age 29; P27, age 41; P23, age 28). The graph of these data indicates a wide variation in the extent of kinetic field in the first two decades of life. Only islands of vision of limited extent were measurable after the third decade of life. 
Limited longitudinal data for kinetic fields are also plotted (Fig. 2A)and illustrated (Figs. 2B 2C 2D) . P8, at age 10 had a full kinetic field (to the V-4e target), but over the ensuing 11 years showed progressive loss of superior and then mid-peripheral fields; at age 21 there was a central island isolated by an absolute scotoma from a temporal peripheral island (Fig. 2B) . P5, at age 10, had generalized constriction of field (39% of normal) and a follow-up at age 17 years revealed only a small central island (Fig. 2C) . P18, at age 21, showed generalized constriction (38% of normal); at age 24, there was a residual central island with a temporal peripheral island (Fig. 2D)
Static threshold perimetry in the dark-adapted state was performed in 17 of the patients. The highest intensity of the white stimulus used in the static perimetry is 1 log unit higher than that in the kinetic perimeter. Maps of dark-adapted sensitivity are shown for normal subjects (mean map of four individuals; age range, 22–61 years) compared with results from eight representative patients with RPE65-LCA. Patients are ordered (left to right in each row) by their mean sensitivity across the field. P14 and P20 had the highest mean sensitivities among the eight patients shown; however, these dark-adapted sensitivities were still approximately 5 log units reduced compared with those of normal subjects (mean normal average, 72 dB [SD, 1.6] versus 23 and 19.1 dB, respectively, for P14 and P20). The sensitivity map for P20 shows some decrement in peripheral sensitivity with relative central and mid-peripheral field preservation. Other dark-adapted sensitivity maps (P11, P8, and P17) show losses in the mid-peripheral field but with residual islands of central and peripheral function. More advanced stages (P21, P13, and P23) show extensive mid-peripheral scotomas separating central from peripheral vision. It is of interest that patients at advanced disease stages with only central islands by kinetic perimetry (n = 4) all showed detectable peripheral islands by dark-adapted static perimetry. The peripheral islands were equal or lower in sensitivity than the central islands. A patient with retained peripheral function but no measurable central function by kinetic perimetry (P23), had measurable central and peripheral islands with dark-adapted static perimetry and there was greater sensitivity in the periphery. Such findings are most likely attributable to the 1-log-unit brighter stimulus available with the static perimeter. 
Dark-adapted perimetry results were summarized by plotting sensitivity as a function of eccentricity, and these cross-sectional data were grouped to arrive at a hypothetical severity sequence of residual visual loss (Fig. 3B) . These data support the notion that widespread loss of sensitivity occurs early in the disease and may progress to patchy loss, which then increases in severity. In normal subjects, sensitivity minimum is at fixation; there is an increase to a peak at ∼12°; and a gradual decline occurs at greater eccentricities. Sensitivity in patients with RPE65-LCA was abnormally reduced at fixation but was still higher than at greater eccentricities, which were at least 4 log units reduced. The different patterns of loss at eccentricities >10° suggest a sequence of severity. At early stages (data from four patients, Fig. 3B , top right), there were relatively homogeneous losses between ∼10° and the periphery. Later stages showed prominent losses between 30° and 60° eccentricity, and these regional mid-peripheral losses deepened while function nearer fixation declined less dramatically (data from five patients, Fig. 3B , lower left). The pattern at even later stages (data from four patients, Fig. 3B , lower right) suggested that the 30° to 60° region of loss had become an absolute scotoma; the extent of this scotoma was greater than at the previous stage and involved more central field. Data from four of these patients of comparable age (19–23 years) were used to illustrate further the hypothesized sequence of residual vision loss in RPE65-LCA (Fig. 3C) . Relatively homogenous loss (P14) was followed by prominent mid-peripheral loss (P8) that can result in an absolute mid-peripheral scotoma (P21); finally, there was centripetal movement of the defect boundary and only central and/or peripheral islands of vision remained (P13). 
Relation of Residual Vision to Residual Photoreceptor Structure
Visual function and retinal structure in RPE65-LCA are related in a complex manner because of dual defects that can affect vision in this disease: a biochemical blockade of the visual cycle and a complicating retinal degenerative process leading to photoreceptor cell loss. 9 18 24 We asked the practical question of whether detectable dark-adapted sensitivity to the white stimulus of the static perimeter had any relationship to the presence of measurable photoreceptor layer (outer nuclear layer, ONL). The answer to this question could be of value in screening candidate patients for therapy and in directing local therapy to appropriate retinal regions, especially those regions in the peripheral retina where large deviations from the optical axis result in loss of signal on OCT scans due to optical distortions. 
Vertical cross-sectional OCT images of the retina spanning approximately 8 mm to either side of the fovea were analyzed in 20 patients with RPE65-LCA for ONL thickness (Fig. 4A) . Vertical profiles of dark-adapted sensitivity were used to relate the presence or absence of visual sensitivity to ONL across this same region. Like the normal subject, P10 at age 12 had detectable visual sensitivity across the vertical meridian. There was a wide extent of measurable ONL (highlighted in blue on scans), although it was substantially reduced in thickness compared with normal. P22 at age 27, had ONL that extended from the fovea to approximately 3 to 4 mm superior and inferior; discontinuous with this ONL was a thinned segment of ONL detectable superiorly. Visual sensitivity was present in most of the region that showed detectable ONL. 
To summarize the data in the 20 patients with RPE65-LCA, we sampled 487 loci along the vertical meridian for ONL thickness and detectable dark-adapted visual sensitivity (Fig. 4B) . There were 95 loci with no measurable vision; 71 of these loci (75%) also had no measurable ONL. The remaining 24 loci with no vision had <13.5 μm of ONL thickness (mean, 8 μm [SD, 3.5]). Among the 392 loci with detectable dark-adapted visual sensitivity, 377 (96%) loci showed measurable ONL (mean, 21 μm [SD, 15]). The conclusion from these data representing a wide central retinal region is that presence of dark-adapted visual sensitivity is highly likely to be associated with the presence of underlying ONL. 
Discussion
Patients with RPE65-LCA in this study and in earlier reports (reviewed in Ref. 16 ) have markedly decreased but residual vision. The consensus from previous studies is that the limited residual function is cone mediated. The present study provides evidence of residual rod as well as cone vision in patients with RPE65-LCA; residual rod function has been reported in studies of Rpe65-deficient mice. 19 22 35 What is the biochemical basis of any residual vision in RPE65-LCA? The most parsimonious answer is that function represents residual RPE65 activity from hypomorphic alleles (i.e., those with reduced but not absent levels of gene activity). In vitro analyses of some of the RPE65 mutant alleles found in patients have indicated that isomerization activity may not be completely lost, suggesting partial function of the visual cycle in vivo. 15 36 37 Consistent with this notion is a report of a relatively mild form of RPE65-LCA in a patient with a mutant allele and in vitro evidence of higher residual levels of RPE65 activity. 38 Further, the Rpe65 R91W knock-in mice, unlike Rpe65 / , have measurable RPE65 and 11-cis-retinal. 21 There remains the possibility, however, that there are alternative RPE65-independent pathways that supply chromophore and are the basis of residual vision. For example, in Rpe65 / mice, there is no measurable 11-cis retinal but definite residual retinal function. 19 It has been determined that 9-cis retinal can accumulate and the rod visual pigment isorhodopsin formed. 22 The exact source of the 9-cis-retinal is unknown, but the level is increased in Rpe65 / mice that are dark reared or have decreased melanin levels. 39 Regeneration of chromophore in cones has long been considered to involve alternative RPE65-independent pathways in addition to the conventional RPE65-dependent visual cycle. 4 17 40  
Patterns of progressive loss of residual vision in RPE65-LCA were estimated with cross-sectional data from kinetic and dark-adapted static perimetry. All patients have at least 3 to 4 log units reduction of sensitivity to light, the presumed consequence of the visual cycle blockade from RPE65 deficiency. If the insensitivity was uniform across the retina, a simple model would predict a sensitivity versus eccentricity plot that resembled the normal (Fig. 3B , upper left) but one that was uniformly reduced by several log units. None of the patients in this study showed exactly this pattern. The mildest pattern did show a relatively slow decline in sensitivities >10°, which resembled the slow decline at these eccentricities in the normal plot. However, these patients also had prominent decreases in sensitivity between fixation and ∼10°. From earlier studies of RPE65-LCA, we know that superimposed on an early-onset biochemical dysfunction is a component of retinal degeneration. 9 17 18 41 Already in the first decade of life, there are cone and rod photoreceptor losses, as demonstrated by measurement of ONL at the fovea and across the central 30° of retina. 17 18 The more central visual losses may at least partly be related to the topography of ONL thinning. 17 18 It is of interest that the mid-peripheral losses in sensitivity mimic patterns of visual field loss in forms of RP, many of which are known to be primary photoreceptor diseases. Late stage patterns with only residual central and peripheral islands are also a common finding in advanced RP. 42 The patterns of residual vision we observed may be partly due to underlying patterns of photoreceptor degeneration, especially at later disease stages. A component of scattered light from stimuli falling on severely degenerate retina may be extending some of the detected islands of vision. Adding further complexity is the possibility that human RPE65-LCA may undergo different rates of cone and rod degeneration, as in murine Rpe65 deficiency. 43  
Our evidence that ONL structure in a wide central region of retina generally follows the residual function, as measured with higher intensity dark-adapted static thresholds, leads to the speculation that such visual data may be usable as a surrogate measure for underlying photoreceptors. The practical implication of this result relates to ongoing clinical trials of gene therapy in RPE65-LCA. 11 12 13 14 The subretinal treatment zone in two of the three clinical trials has been mainly macular. 11 12 There is not yet any proof of efficacy in terms of foveal visual acuity and the occurrence of a complicating macular hole certainly indicates that foveomacular injections carry some increased complication risks. 12 We suggest that perifoveal or mid-peripheral subretinal injection sites be considered as alternate targets for gene therapy based on our recent OCT studies 17 18 and the present results indicating mid-peripheral preservation of residual sensitivity at relatively early disease stages. For patients at later disease stages, the choices become limited. These patients may be relegated to a category of ineligible for participation in gene therapy trials. Alternatively, if regions in their peripheral retina are functioning, it may be worth considering such patients for treatment. The only way to determine the value of this approach may be to perform peripheral retinal gene therapy in these patients. Such regions are less accessible to OCT because large deviations from the optical axis during imaging cause distortions and loss of signal. With the goal of enhancing orientation and mobility in patients who would not be strong candidates for more centrally located focal treatment, we propose that retained temporal peripheral vision responding to dark-adapted high intensity stimuli should be considered as an eligibility criterion for gene therapy in the nasal retina. The concept may be generalizable in the future for treatment of the many forms of RP with retained peripheral visual islands. 
 
Table 1.
 
Molecular and Clinical Characteristics of the RPE65-LCA Patients
Table 1.
 
Molecular and Clinical Characteristics of the RPE65-LCA Patients
Patient Age at First Visit (y)/Sex Ethnicity Mutations Visual Acuity (RE-LE)* Fundus Features, † Ages at Follow-up Visits (y) Reference, ‡
P1, § 4/M Indian A500del5bp/A500del5bp 20/100 17
P2, § 5/F Indian A500del5bp/A500del5bp 20/125 17
P3, ∥ 6/M Indian R44Q/R44Q 20/63 17 18
P4 7/F Black R91W/R91W 20/63 , ¶ 17 18
P5 7/F Hispanic 97del20bp/97del20bp 20/160 10, 12, 17 9 17 18 23 24
P6, ∥ 7/M Indian R44Q/R44Q 20/160 17 18
P7, # 7/M Hispanic L341S/IVS2-2A>C 20/100-20/200 10 18
P8 10/M Caucasian Y368H/Y368H 20/160-20/100 11, 13, 19, 20, 21 9 17 23
P9 6/F Black L408P/L408P 20/80-20/50 12 17 18
P10, # 9/M Hispanic L341S/IVS2-2A>C 20/63-20/80 12 18
P11 13/F Indian V287F/V287F 20/125-20/200 17 18
P12 14/F Caucasian R91Q/R91W 20/32-20/32 17 18
P13 18/F Hispanic L341S/L341S 20/250-20/320 20,21 9 17
P14 19/F Caucasian G40S/R91Q 20/320-20/400 20 17 18 24
P15, ** 19/F Black-Indian R91Q/IVS7+4A>G 20/400 31 17
P16 19/M Black R91W/R91W 20/200-20/800 21 17 24
P17 19/F White R91W/R44Q 20/200-20/160 22, 23, 24 9 17
P18 21/M White E417Q/E417Q 20/160 23,24,25 9 17
P19, ** 22/M Black-Indian R91Q/IVS7+4A>G 20/200-20/70 This study
P20 23/M Asian R91W/1059_1060ins1bp 20/60-20/40 17 18 24
P21 23/F Caucasian G104D/G40S 20/125-20/160 , †† This study
P22 27/F Asian H182R/H182R 20/160-20/1600 9 17
P23 28/F Caucasian Y368H/297del1bp LP 31 9 17
P24 29/M Caucasian H182Y/G40S 20/800-20/640 , ††, , ‡‡ This study
P25 33/F Caucasian IVS1+5G>A/W460X 20/1600-20/800 This study
P26 35/M Caucasian IVS1+5G>A homoallelic 20/1600-20/800 , ††, , ‡‡ 37,41,44,47 9 17
P27 36/M Caucasian Y144D/Y144D 20/200 , ‡‡ 41 9 17
P28 40/F Caucasian K303X/Y431C HM-20/1600 , ‡‡ 9 17
P29 46/F Caucasian Y239D/Y368H LP , ‡‡ This study
P30 55/M Caucasian A132T/A132T LP , ††, , ‡‡ This study
Figure 1.
 
Measures of residual function in RPE65-LCA. (A) Standard ERGs in patients with RPE65-LCA. Rod, mixed cone–rod, and cone ERGs from six representative patients with RPE65-LCA (age range, 5–23 years) were compared with ERGs of a patient with a rhodopsin (R135L) gene mutation showing residual, severely abnormal, cone-mediated function. A normal subject (age 20 years) is shown for comparison (left). Traces start at stimulus onset; calibrations are to the right and below waveforms. ERGs can be undetectable, even at early ages. Detectable ERGs show a pattern similar to that of the patient with a RHO mutation and severe rod dysfunction but residual and abnormal cone function. (B) Inset (left): FST sensitivity loss to a white stimulus in patients with RPE65-LCA ranked by age. Chromatic FST sensitivity differences (blue-red) in patients with RPE65-LCA ranked in decreasing order of magnitude (right). Results in normal subjects in the dark-adapted state (left) or at the cone plateau of dark-adaptation after light-exposure (right) served to define which photoreceptor mediates perception of each color (error bars, mean ± 2 SD). Labels above the bars denote photoreceptor mediation: R, rods; M, mixed; C, cones. Ages of the patients and their numbers are shown below each bar on the horizontal axis. Dashed line: delimits the upper limit for categorization as cone-mediated.
Figure 1.
 
Measures of residual function in RPE65-LCA. (A) Standard ERGs in patients with RPE65-LCA. Rod, mixed cone–rod, and cone ERGs from six representative patients with RPE65-LCA (age range, 5–23 years) were compared with ERGs of a patient with a rhodopsin (R135L) gene mutation showing residual, severely abnormal, cone-mediated function. A normal subject (age 20 years) is shown for comparison (left). Traces start at stimulus onset; calibrations are to the right and below waveforms. ERGs can be undetectable, even at early ages. Detectable ERGs show a pattern similar to that of the patient with a RHO mutation and severe rod dysfunction but residual and abnormal cone function. (B) Inset (left): FST sensitivity loss to a white stimulus in patients with RPE65-LCA ranked by age. Chromatic FST sensitivity differences (blue-red) in patients with RPE65-LCA ranked in decreasing order of magnitude (right). Results in normal subjects in the dark-adapted state (left) or at the cone plateau of dark-adaptation after light-exposure (right) served to define which photoreceptor mediates perception of each color (error bars, mean ± 2 SD). Labels above the bars denote photoreceptor mediation: R, rods; M, mixed; C, cones. Ages of the patients and their numbers are shown below each bar on the horizontal axis. Dashed line: delimits the upper limit for categorization as cone-mediated.
Figure 2.
 
Kinetic perimetry in RPE65-LCA. (A) Kinetic field extent expressed as a percentage of normal and plotted as a function of age of patient. Longitudinal data are connected by lines. Representative kinetic fields illustrating early and later stage patterns are shown (above and to the right of the graph). All fields are depicted as right eyes. (BD) Serial kinetic fields in one eye of three patients spanning 11 years in P8 (B), 7 years in P5 (C), and 3 years in P18 (D). Patients with illustrated visual fields are identified in (A).
Figure 2.
 
Kinetic perimetry in RPE65-LCA. (A) Kinetic field extent expressed as a percentage of normal and plotted as a function of age of patient. Longitudinal data are connected by lines. Representative kinetic fields illustrating early and later stage patterns are shown (above and to the right of the graph). All fields are depicted as right eyes. (BD) Serial kinetic fields in one eye of three patients spanning 11 years in P8 (B), 7 years in P5 (C), and 3 years in P18 (D). Patients with illustrated visual fields are identified in (A).
Figure 3.
 
Dark-adapted static threshold perimetry to a white stimulus in RPE65-LCA. (A) Sensitivities at 71 loci in normal subjects (N) and patients with RPE65-LCA are mapped to a pseudocolor scale representing 7 log units. Eight patient sensitivity maps are shown and ordered (left to right in each of three rows) by mean sensitivity calculated across the field. All data are depicted as right eyes to enable comparison. The normal blind spot is shown as a black square at the 12° temporal field. (B) Sensitivity as a function of eccentricity in patients with RPE65-LCA compared with normal subjects (top left). Patients are grouped by increasing severity of sensitivity loss (from top right to lower left to lower right; and within panels from top to bottom). Data traces are colored to show the two decades of ages represented (orange, 10–19 years; purple, 20–29 years). (C) Data from four patients of comparable age (19–23 years) that illustrate further the patterns of increasing severity.
Figure 3.
 
Dark-adapted static threshold perimetry to a white stimulus in RPE65-LCA. (A) Sensitivities at 71 loci in normal subjects (N) and patients with RPE65-LCA are mapped to a pseudocolor scale representing 7 log units. Eight patient sensitivity maps are shown and ordered (left to right in each of three rows) by mean sensitivity calculated across the field. All data are depicted as right eyes to enable comparison. The normal blind spot is shown as a black square at the 12° temporal field. (B) Sensitivity as a function of eccentricity in patients with RPE65-LCA compared with normal subjects (top left). Patients are grouped by increasing severity of sensitivity loss (from top right to lower left to lower right; and within panels from top to bottom). Data traces are colored to show the two decades of ages represented (orange, 10–19 years; purple, 20–29 years). (C) Data from four patients of comparable age (19–23 years) that illustrate further the patterns of increasing severity.
Figure 4.
 
Relationship between dark-adapted visual function and retinal structure in RPE65-LCA. (A) Vertical cross-sectional retinal images using OCT compared with the presence or absence of visual response in corresponding locations. A 48-year-old normal subject and two patients with RPE65-LCA (P10, P22) are compared. Each patient shows a different degree of ONL preservation (highlighted in blue on scan). Apparent peaks at the vitreoretinal surface at ∼4 to 5 mm eccentricity along some of these vertical scans are the nerve fiber layer bundles and arcade vessels. (B) Summary of data from 487 loci along the vertical meridian in 20 patients. ONL thickness is plotted for loci with absence (left, 95 loci) or presence (right, 392 loci) of dark-adapted visual sensitivity.
Figure 4.
 
Relationship between dark-adapted visual function and retinal structure in RPE65-LCA. (A) Vertical cross-sectional retinal images using OCT compared with the presence or absence of visual response in corresponding locations. A 48-year-old normal subject and two patients with RPE65-LCA (P10, P22) are compared. Each patient shows a different degree of ONL preservation (highlighted in blue on scan). Apparent peaks at the vitreoretinal surface at ∼4 to 5 mm eccentricity along some of these vertical scans are the nerve fiber layer bundles and arcade vessels. (B) Summary of data from 487 loci along the vertical meridian in 20 patients. ONL thickness is plotted for loci with absence (left, 95 loci) or presence (right, 392 loci) of dark-adapted visual sensitivity.
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Figure 1.
 
Measures of residual function in RPE65-LCA. (A) Standard ERGs in patients with RPE65-LCA. Rod, mixed cone–rod, and cone ERGs from six representative patients with RPE65-LCA (age range, 5–23 years) were compared with ERGs of a patient with a rhodopsin (R135L) gene mutation showing residual, severely abnormal, cone-mediated function. A normal subject (age 20 years) is shown for comparison (left). Traces start at stimulus onset; calibrations are to the right and below waveforms. ERGs can be undetectable, even at early ages. Detectable ERGs show a pattern similar to that of the patient with a RHO mutation and severe rod dysfunction but residual and abnormal cone function. (B) Inset (left): FST sensitivity loss to a white stimulus in patients with RPE65-LCA ranked by age. Chromatic FST sensitivity differences (blue-red) in patients with RPE65-LCA ranked in decreasing order of magnitude (right). Results in normal subjects in the dark-adapted state (left) or at the cone plateau of dark-adaptation after light-exposure (right) served to define which photoreceptor mediates perception of each color (error bars, mean ± 2 SD). Labels above the bars denote photoreceptor mediation: R, rods; M, mixed; C, cones. Ages of the patients and their numbers are shown below each bar on the horizontal axis. Dashed line: delimits the upper limit for categorization as cone-mediated.
Figure 1.
 
Measures of residual function in RPE65-LCA. (A) Standard ERGs in patients with RPE65-LCA. Rod, mixed cone–rod, and cone ERGs from six representative patients with RPE65-LCA (age range, 5–23 years) were compared with ERGs of a patient with a rhodopsin (R135L) gene mutation showing residual, severely abnormal, cone-mediated function. A normal subject (age 20 years) is shown for comparison (left). Traces start at stimulus onset; calibrations are to the right and below waveforms. ERGs can be undetectable, even at early ages. Detectable ERGs show a pattern similar to that of the patient with a RHO mutation and severe rod dysfunction but residual and abnormal cone function. (B) Inset (left): FST sensitivity loss to a white stimulus in patients with RPE65-LCA ranked by age. Chromatic FST sensitivity differences (blue-red) in patients with RPE65-LCA ranked in decreasing order of magnitude (right). Results in normal subjects in the dark-adapted state (left) or at the cone plateau of dark-adaptation after light-exposure (right) served to define which photoreceptor mediates perception of each color (error bars, mean ± 2 SD). Labels above the bars denote photoreceptor mediation: R, rods; M, mixed; C, cones. Ages of the patients and their numbers are shown below each bar on the horizontal axis. Dashed line: delimits the upper limit for categorization as cone-mediated.
Figure 2.
 
Kinetic perimetry in RPE65-LCA. (A) Kinetic field extent expressed as a percentage of normal and plotted as a function of age of patient. Longitudinal data are connected by lines. Representative kinetic fields illustrating early and later stage patterns are shown (above and to the right of the graph). All fields are depicted as right eyes. (BD) Serial kinetic fields in one eye of three patients spanning 11 years in P8 (B), 7 years in P5 (C), and 3 years in P18 (D). Patients with illustrated visual fields are identified in (A).
Figure 2.
 
Kinetic perimetry in RPE65-LCA. (A) Kinetic field extent expressed as a percentage of normal and plotted as a function of age of patient. Longitudinal data are connected by lines. Representative kinetic fields illustrating early and later stage patterns are shown (above and to the right of the graph). All fields are depicted as right eyes. (BD) Serial kinetic fields in one eye of three patients spanning 11 years in P8 (B), 7 years in P5 (C), and 3 years in P18 (D). Patients with illustrated visual fields are identified in (A).
Figure 3.
 
Dark-adapted static threshold perimetry to a white stimulus in RPE65-LCA. (A) Sensitivities at 71 loci in normal subjects (N) and patients with RPE65-LCA are mapped to a pseudocolor scale representing 7 log units. Eight patient sensitivity maps are shown and ordered (left to right in each of three rows) by mean sensitivity calculated across the field. All data are depicted as right eyes to enable comparison. The normal blind spot is shown as a black square at the 12° temporal field. (B) Sensitivity as a function of eccentricity in patients with RPE65-LCA compared with normal subjects (top left). Patients are grouped by increasing severity of sensitivity loss (from top right to lower left to lower right; and within panels from top to bottom). Data traces are colored to show the two decades of ages represented (orange, 10–19 years; purple, 20–29 years). (C) Data from four patients of comparable age (19–23 years) that illustrate further the patterns of increasing severity.
Figure 3.
 
Dark-adapted static threshold perimetry to a white stimulus in RPE65-LCA. (A) Sensitivities at 71 loci in normal subjects (N) and patients with RPE65-LCA are mapped to a pseudocolor scale representing 7 log units. Eight patient sensitivity maps are shown and ordered (left to right in each of three rows) by mean sensitivity calculated across the field. All data are depicted as right eyes to enable comparison. The normal blind spot is shown as a black square at the 12° temporal field. (B) Sensitivity as a function of eccentricity in patients with RPE65-LCA compared with normal subjects (top left). Patients are grouped by increasing severity of sensitivity loss (from top right to lower left to lower right; and within panels from top to bottom). Data traces are colored to show the two decades of ages represented (orange, 10–19 years; purple, 20–29 years). (C) Data from four patients of comparable age (19–23 years) that illustrate further the patterns of increasing severity.
Figure 4.
 
Relationship between dark-adapted visual function and retinal structure in RPE65-LCA. (A) Vertical cross-sectional retinal images using OCT compared with the presence or absence of visual response in corresponding locations. A 48-year-old normal subject and two patients with RPE65-LCA (P10, P22) are compared. Each patient shows a different degree of ONL preservation (highlighted in blue on scan). Apparent peaks at the vitreoretinal surface at ∼4 to 5 mm eccentricity along some of these vertical scans are the nerve fiber layer bundles and arcade vessels. (B) Summary of data from 487 loci along the vertical meridian in 20 patients. ONL thickness is plotted for loci with absence (left, 95 loci) or presence (right, 392 loci) of dark-adapted visual sensitivity.
Figure 4.
 
Relationship between dark-adapted visual function and retinal structure in RPE65-LCA. (A) Vertical cross-sectional retinal images using OCT compared with the presence or absence of visual response in corresponding locations. A 48-year-old normal subject and two patients with RPE65-LCA (P10, P22) are compared. Each patient shows a different degree of ONL preservation (highlighted in blue on scan). Apparent peaks at the vitreoretinal surface at ∼4 to 5 mm eccentricity along some of these vertical scans are the nerve fiber layer bundles and arcade vessels. (B) Summary of data from 487 loci along the vertical meridian in 20 patients. ONL thickness is plotted for loci with absence (left, 95 loci) or presence (right, 392 loci) of dark-adapted visual sensitivity.
Table 1.
 
Molecular and Clinical Characteristics of the RPE65-LCA Patients
Table 1.
 
Molecular and Clinical Characteristics of the RPE65-LCA Patients
Patient Age at First Visit (y)/Sex Ethnicity Mutations Visual Acuity (RE-LE)* Fundus Features, † Ages at Follow-up Visits (y) Reference, ‡
P1, § 4/M Indian A500del5bp/A500del5bp 20/100 17
P2, § 5/F Indian A500del5bp/A500del5bp 20/125 17
P3, ∥ 6/M Indian R44Q/R44Q 20/63 17 18
P4 7/F Black R91W/R91W 20/63 , ¶ 17 18
P5 7/F Hispanic 97del20bp/97del20bp 20/160 10, 12, 17 9 17 18 23 24
P6, ∥ 7/M Indian R44Q/R44Q 20/160 17 18
P7, # 7/M Hispanic L341S/IVS2-2A>C 20/100-20/200 10 18
P8 10/M Caucasian Y368H/Y368H 20/160-20/100 11, 13, 19, 20, 21 9 17 23
P9 6/F Black L408P/L408P 20/80-20/50 12 17 18
P10, # 9/M Hispanic L341S/IVS2-2A>C 20/63-20/80 12 18
P11 13/F Indian V287F/V287F 20/125-20/200 17 18
P12 14/F Caucasian R91Q/R91W 20/32-20/32 17 18
P13 18/F Hispanic L341S/L341S 20/250-20/320 20,21 9 17
P14 19/F Caucasian G40S/R91Q 20/320-20/400 20 17 18 24
P15, ** 19/F Black-Indian R91Q/IVS7+4A>G 20/400 31 17
P16 19/M Black R91W/R91W 20/200-20/800 21 17 24
P17 19/F White R91W/R44Q 20/200-20/160 22, 23, 24 9 17
P18 21/M White E417Q/E417Q 20/160 23,24,25 9 17
P19, ** 22/M Black-Indian R91Q/IVS7+4A>G 20/200-20/70 This study
P20 23/M Asian R91W/1059_1060ins1bp 20/60-20/40 17 18 24
P21 23/F Caucasian G104D/G40S 20/125-20/160 , †† This study
P22 27/F Asian H182R/H182R 20/160-20/1600 9 17
P23 28/F Caucasian Y368H/297del1bp LP 31 9 17
P24 29/M Caucasian H182Y/G40S 20/800-20/640 , ††, , ‡‡ This study
P25 33/F Caucasian IVS1+5G>A/W460X 20/1600-20/800 This study
P26 35/M Caucasian IVS1+5G>A homoallelic 20/1600-20/800 , ††, , ‡‡ 37,41,44,47 9 17
P27 36/M Caucasian Y144D/Y144D 20/200 , ‡‡ 41 9 17
P28 40/F Caucasian K303X/Y431C HM-20/1600 , ‡‡ 9 17
P29 46/F Caucasian Y239D/Y368H LP , ‡‡ This study
P30 55/M Caucasian A132T/A132T LP , ††, , ‡‡ This study
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