Penetrating keratoplasty (PK) involves replacement of host stroma and endothelium by donor tissue and requires transection of all host corneal nerves. Changes in the endothelium after PK are well documented and include a faster-than-normal rate of cell loss^1,2 and decreased permeability.³ Chronic endothelial dysfunction after PK has been associated with stromal haze, and, collectively, these findings constitute late endothelial failure (LEF),^4,5 which is the leading cause of graft failure.^1,2

The etiology of stromal haze in LEF is not known, but changes in keratocyte density and function, or in the extracellular matrix, might increase corneal backscatter. Little is known about the role of keratocytes and corneal nerves after PK and whether changes in these cell populations affect graft clarity. Confocal microscopy enables visualization of stromal keratocytes and corneal nerve fiber bundles in vivo, and we have devised methods for quantifying keratocyte density and subbasal nerve fiber density from confocal images of corneas.^6–8 In a preliminary study that used this method, we found that keratocyte density was decreased in clear penetrating grafts compared to normal corneas.⁹ In the present study, we expanded our series of clear penetrating grafts and also report keratocyte and subbasal nerve densities in grafts with LEF.

Ninety-nine clear grafts in 74 patients and 21 grafts with LEF in 19 patients were enrolled. Sixty-three normal (unoperated) corneas of 63 subjects who were enrolled in 3 other studies conducted between 2000 and 2006 were used as concurrent controls for keratocyte density,^10–12 and 76 normal corneas of 76 different subjects enrolled in 2 studies conducted in 1998 were used as controls for subbasal nerve density.^8,13 The annual rate of change of keratocytes was estimated from clear grafts examined at least 5 years after PK on 2 occasions separated by 4 or more years.

TABLE 1 PREOPERATIVE DIAGNOSES IN CLEAR GRAFTS AND GRAFTS WITH LATE ENDOTHELIAL FAILURE

TABLE 2 KERATOCYTE DENSITY AND NUMBER OF KERATOCYTES IN NORMAL CORNEAS, CLEAR GRAFTS, AND GRAFTS WITH LATE ENDOTHELIAL FAILURE (MEAN ± STANDARD DEVIATION)

FIGURE 1 Keratocyte density in normal (unoperated) corneas, clear penetrating grafts, and grafts with late endothelial failure (LEF) is shown as a function of stromal depth. Keratocyte densities in all layers of the stroma after penetrating keratoplasty (clear (more ...)

FIGURE 2 Confocal microscopy image of subbasal nerve fiber bundle 26 years after penetrating keratoplasty. Subbasal nerve fiber bundles were not detected in 48% of clear grafts, but when regeneration was evident, nerve fiber bundles were often tortuous and disordered. (more ...)

Mean keratocyte density correlated weakly with time after PK (r = −0.20, P = .05, n = 99), whereas there was no correlation between the number of keratocytes and time after PK (r = −0.04, P = .68, n = 99, Figure 3, Table 3). Correlations between keratocyte density in each layer and time after PK are shown in Table 3. Stromal thickness correlated with time after PK (r = 0.26, P = .009, n = 99). Recovery of subbasal nerve density also correlated with time after PK (r = 0.36, P < .001, n = 94, Table 3, Figure 4).

FIGURE 3 Relationship between number of keratocytes and time after penetrating keratoplasty (PK). Cross-sectional analysis of 99 clear penetrating grafts revealed no correlation between the number of keratocytes in the full-thickness central stroma with time after (more ...)

TABLE 3 CORRELATIONS WITH TIME AFTER KERATOPLASTY IN CLEAR GRAFTS*

FIGURE 4 Relationship between subbasal nerve fiber bundle density and time after penetrating keratoplasty (PK). Cross-sectional analysis of 94 clear penetrating grafts suggested that subbasal nerve fiber bundle density increased with time after PK (r = 0.36, (more ...)

Sixteen clear grafts of 14 eyes were examined on 2 occasions separated by 5.0 ± 0.6 years (range, 4–6 years). The first examination was 17.6 ± 4.8 years after keratoplasty (range, 5–24 years), and the second examination was 22.6 ± 5.2 years after keratoplasty (range, 9–30 years). The preoperative diagnosis was keratoconus in 13 eyes and Fuchs dystrophy in 3 eyes. Mean keratocyte density for the full-thickness stroma was decreased 13% at the later examination compared to the earlier examination (P = .02, Table 4). Keratocyte density decreased only in the middle and posterior thirds of the stroma between the earlier and later examinations (Table 4, Figure 5). The number of keratocytes was decreased 13% at the later examination compared to the earlier examination (P = .03, Table 4). The rate of loss of keratocytes was 2.9 ± 5.0% per year. Central stromal thickness did not differ between the earlier (461 ± 40 μm) and later (473 ± 61 μm) examinations (P = .48); the minimum detectable difference was 50 μm (α = .05, β = .20, n = 16).

TABLE 4 KERATOCYTE DENSITY AT REPEATED EXAMINATIONS OF CLEAR PENETRATING GRAFTS (MEAN ± STANDARD DEVIATION)*

FIGURE 5 Keratocyte density at repeated examinations of clear penetrating grafts. Sixteen clear grafts of 14 patients were examined twice ≥ 4 years apart and ≥ 5 years after penetrating keratoplasty. The first examination was 17.6 ± 4.8 (more ...)

FIGURE 6 Anterior keratocytes in late endothelial failure (LEF). Confocal microscopy image of anterior keratocytes in a penetrating graft with LEF shows visible cell processes, suggesting activation of keratocytes and preventing identification of individual cells (more ...)

Keratocyte density and keratocyte number per mm² of full-thickness stroma did not differ between grafts with LEF and clear grafts (Table 2, Figure 1). The central stroma in grafts with LEF (508 ± 48 μm) was thicker than in clear grafts (470 ± 46 μm, P = .008). Median subbasal nerve density in grafts with LEF (340 μm/mm², n = 11) did not differ from clear grafts (150 μm/mm², n = 94, P = .95).

Keratocyte density and subbasal nerve fiber bundle density after PK were significantly lower than in normal corneas when measured by using confocal microscopy in vivo. Although keratocytes after PK were lost at a faster-than-normal rate,⁶ we were unable to detect a difference between keratocyte density in clear grafts compared to grafts with LEF. Subbasal nerve fiber bundles did not appear to regenerate to any clinically significant extent through 30 years after PK.

In normal corneas, keratocyte density is highest in the most anterior layers of the stroma, and full-thickness density declines with age at a rate similar to normal corneal endothelial and trabecular meshwork cells.⁶ Given that central corneal thickness increases with time after keratoplasty^1,2 and that in the present study, the stroma of penetrating grafts was thicker than normal, it is not surprising that keratocyte density in clear grafts was decreased compared to normal because of redistribution of cells over a larger volume of stroma. However, we also calculated the absolute number of keratocytes in a column of full-thickness stroma, and we confirmed our preliminary report that the number of keratocytes was reduced in penetrating grafts compared to normal, contributing to decreased keratocyte density.⁹ Paired analysis showed that the number of keratocytes in the central stroma continued to decrease many years after keratoplasty at a rate of 2.9 ± 5.0% per year. Keratocyte density therefore also decreased over the 5-year period, but only in the middle and posterior thirds of the cornea. The latter can be explained by the posterior stroma swelling more than the anterior stroma,²⁰ and although we did not detect an increase in stromal thickness over the 5-year period between repeated examinations, with the sample size, we were unable to detect differences smaller than 50 μm. The rate of decrease of keratocytes of 2.9% per year in the paired analysis was not supported by the cross-sectional analysis (Figure 3) and was much higher than the rate of endothelial cell loss in the second decade after keratoplasty.^1,2 We analyzed confocal image contrast between the first and second examinations in the paired analysis and found that contrast was significantly lower at the second examination compared to the first examination. However, even after adjusting keratocyte density for variations in contrast, keratocyte density and the number of keratocytes were still 10% lower at the second examination compared to the first examination. We are unaware of other studies that have quantified keratocyte loss after PK, but it is conceivable that keratocytes are lost at a faster rate than endothelial cells and that keratocyte loss is higher within certain subgroups after PK.

Donor keratocytes are lost by apoptosis and necrosis during tissue preservation,²¹ but continued keratocyte losses several years after transplantation have not been previously documented. Keratocyte loss in penetrating grafts might be caused by starvation from decreased endothelial permeability,³ chronic apoptosis,²² or other undefined mechanisms, and may result in a gradual decrease in corneal transparency. Although we were unable to detect a difference in the number of keratocytes between grafts with LEF (with decreased transparency) and clear grafts, this study had limited power to detect small differences, was cross-sectional and not prospective in design, and the sample may have been biased because only 12 of 21 grafts with LEF had images that could be analyzed quantitatively. Because clear grafts lost keratocytes years after keratoplasty, grafts with LEF, which were examined longer after keratoplasty than the clear grafts, would have been expected to have a lower number of keratocytes, possibly contributing to decreased stromal clarity. Histologic analysis of excised grafts for LEF will help to confirm or refute the latter hypothesis.

In clear penetrating grafts, it is unclear whether transplanted keratocytes survive for decades or whether they are replaced by host keratocytes that migrate from the periphery. Donor keratocytes survive in clear grafts for at least a year after keratoplasty in rabbits^23,24 and for as long as 4 years after keratoplasty in failed grafts in humans.²⁵ Keratocytes also have migratory potential and can repopulate epikeratophakia lenticules,^26–29 anterior lamellar grafts,³⁰ and acellular collagen implants.³¹ Our study was not designed to determine whether host keratocytes migrate into the donor, but if that were the case, the results indicate that the rate of repopulation would be inadequate to maintain or increase the number of keratocytes in the corneal stroma.

Alterations in stromal transparency after PK could result from keratocyte dysfunction with or without decreased keratocyte density. The transparency of keratocytes appears to be related to the expression of intracellular crystallins, and decreased crystallin expression has been associated with repair cell phenotypes and increased backscatter from cells.^32,33 We frequently noted keratocyte activation in grafts with LEF (Figure 6), and chronic keratocyte activation after PK might result in increased corneal backscatter,³⁴ which would clinically manifest as stromal translucency. Evaluation of grafts excised for LEF may help determine whether keratocyte dysfunction and altered levels of crystallin expression are associated with LEF.

Decreased keratocyte density after PK has been found by other investigators using different confocal microscopes. Hollingsworth and colleagues³⁵ used a scanning slit confocal microscope and found that anterior and posterior keratocyte densities were decreased but stable over the first year after keratoplasty compared to normal corneas, similar to our prospective data during the first year after PK.⁹ Niederer and colleagues³⁶ used a laser scanning confocal microscope and found that keratocyte density was decreased in the anterior, middle, and posterior thirds of penetrating grafts several years after keratoplasty. The confocal microscopes used in the 2 latter studies are limited in their ability to measure the depth of confocal images accurately, and therefore volumetric keratocyte density and the absolute number of keratocytes were not calculated, preventing direct comparison to our study. However, the confocal microcopy images in the studies by Hollingsworth and colleagues and by Niederer and colleagues are of higher contrast compared to images from our Tandem Scanning confocal microscope, and identifying objects as keratocytes is easier than with our system. Nevertheless, Mikek and colleagues³⁷ also used a scanning slit confocal microscope with high contrast images and found no difference in keratocyte density after PK compared to normal corneas. Because interpretation of the low contrast images from our confocal microscope can be subjective, we used an automated program to identify keratocytes objectively and calculate keratocyte density.¹⁶

Subbasal nerve fiber bundles are transected during PK, and regeneration of nerve fiber bundles in the donor is slow and incomplete, even 3 decades after surgery. In fact, no subbasal nerve fiber bundles could be detected in almost half of the clear grafts that were examined. Our cross-sectional data suggest an increase in subbasal nerve density with time after keratoplasty, but the increase was not clinically significant in the context of normal subbasal nerve density. Slow and limited subbasal nerve regeneration after PK in humans has been previously demonstrated by using confocal microscopy^36,38 and by using acetylcholinesterase staining ex vivo.³⁹ Corneal sensation was not measured in the present study, but sensitivity is known to remain significantly reduced, if not absent, for decades after PK.^40–42 Tervo and colleagues³⁹ showed that epithelial innervation was re-established after PK in humans, but stromal nerve regeneration was essentially absent, and they suggested that the discontinuity of Schwann cell channels at the graft-host junction impaired stromal nerve regeneration. Indeed, Tervo’s hypothesis is supported by evidence of significant stromal nerve regeneration after close apposition of limbal incisions in rabbits,⁴³ and also by recovery of normal subbasal nerve density by 2 and 5 years after photorefractive keratectomy and laser in situ keratomileusis, respectively.^13,44–46 The reason for higher subbasal nerve density in grafts for keratoconus compared to grafts for Fuchs dystrophy is not known, but our results confirm the findings of Niederer and colleagues.³⁶

Whether corneal nerves are required to sustain keratocyte density and function is uncertain, but anterior keratocyte losses have been noted after keratorefractive surgery, in which there is an extended period of denervation postoperatively.^13,45,47 No specific physiologic relationships between nerves and keratocytes have been established, but anatomically, human corneal nerve fibers invaginate the cytoplasm of keratocytes, suggesting that keratocytes might receive trophic factors from corneal nerves.¹⁷ After PK, chronic graft denervation might contribute to keratocyte loss or dysfunction and subsequent decreased transparency.

Further studies are necessary to determine the mechanisms of keratocyte loss after PK and the relationships between corneal nerves, keratocytes, endothelial cells, and stromal transparency. Preventing loss of stromal transparency could improve graft longevity. Furthermore, similar physiologic processes might affect the transparency of the host stroma after posterior lamellar keratoplasty, which is currently popular among corneal surgeons,⁴⁸ and could affect the long-term success of these procedures.

The corneal keratocytes make up 3% to 5% of the total stromal volume in normal eyes¹ and have a higher density in the layers just below the epithelium.² They secrete proteoglycans, collagen, and proteases and appear to be responsible for some of the embryologic stromal deposition and have a major role in stromal wound healing.³ The keratocytes’ role in normal corneal health is not well understood. This is also true of postsurgical (PK, PRK, LASIK) eyes.^4,5

This study adds to our knowledge of the potential role of keratocytes in late endothelial failure (LEF). Since the number of keratocytes decreases over time in both normal and post keratoplasty (PK) eyes, does this decrease cause the endothelium to fail? This study shows that there is no significant difference in the density of keratocytes between normal and LEF eyes. Also, this study confirms previous studies that show a marked decrease in corneal innervation after PK. Forty-five clear grafts (48%) did not have any detectable innervation. The authors do not report if the number corneal nerves have any relationship to the number of keratocytes present in PK eyes.

There are a few weaknesses in this study, which the authors acknowledge. There was limited clinical material available for study, especially for longitudinal measurements. Also, in only 12 of 21 LEF eyes were reliable keratocyte densities measurable.

IT equipment and automated analysis software used in this study is not readily available for confirmatory studies. I would hope that the authors would work with the equipment manufacturers to make this important type of clinical analysis part of routine practice. Dr Bourne’s early work in endothelial analysis led to this measurement becoming a standard in corneal evaluations.

Financial Disclosures: None.

Funding/Support: Supported in part by grant EY 02037 from the National Institutes of Health; Research to Prevent Blindness, Inc (S.V.P. as Olga Keith Wiess Scholar and an unrestricted grant to the Department of Ophthalmology, Mayo Clinic); and the Mayo Foundation.

Financial Disclosures: None.

Author Contributions: Design and conduct of the study (S.V.P., J.C.E, J.W.M, W.M.B.); Collection, management, analysis, and interpretation of the data (S.V.P., J.C.E, J.W.M, W.M.B.); Preparation, review, and approval of the manuscript (S.V.P., J.C.E, J.W.M, W.M.B.).