In Vivo Confocal Microscopy in Limbal Stem Cell Deficiency After Mesenchymal Stem Cell Transplantation: A Sub-analysis from a Phase I–II Clinical Trial

The Heidelberg Retinal Tomograph version 3 (HRT3) with a Rostock cornea module (RCM) (RCM-HRT3) (Heidelberg GmbH, Heidelberg, Germany) was used to analyze the corneal and limbal areas before and after transplantation. Disposable and sterile contact caps (TomoCap^® Heidelberg GmbH) were used to allow contact between the cornea and the objective lens of the IVCM. A lubricating gel (Viscotears^® 0.2% with Carbomero 980; Novartis, Basel, Switzerland) was used to cover and fill the corneal contact caps. Also, topical anesthesia (tetracaine 0.1% and oxybuprocaine 0.4%; Alcon Cusí, Barcelona, Spain) was used prior to IVCM image acquisition. High-contrast digital images with a field of view of 400 × 400 μm (0.16 mm²) were acquired. The transverse resolution and thickness of the optical sections were 2 and 4 μm, respectively. Sequential scans of the central cornea and superior, inferior, temporal, and nasal limbus (12, 3, 6, 9 o’clock positions) using the manual frame acquisition technique were obtained following methods previously described [13, 20]. A minimum of 40 z-scan images were visualized at each examination point from the epithelium to the stroma in the central cornea, or to the palisades of Vogt in the limbus. To increase the likelihood of assessing the same location, external fixation targets were presented to the contralateral eye—one distance target for the central cornea and four eccentric ones for each quadrant of the limbus. Central cornea scans were performed to assess the phenotype of the central epithelium. Cell morphology was classified as corneal, conjunctival, or mixed-type depending on the IVCM findings [30, 31]. When classifying the central phenotype, corneal epithelium was considered as a multi-layered anatomical structure having polygonal and flat cells with hyperreflective nuclei in the superficial layer, progressively decreasing in size in the intermediate layers, and small cells without detectable nuclei with reflective borders in the basal layer [32]; and the conjunctival epithelium as a stratified anatomical structure of cuboidal or polygonal cells having hyporeflective cytoplasm with or without detectable nuclei, and barely defined borders [30, 33]. Limbal scans were performed to assess the presence or absence of palisades of Vogt and the morphologic transition of epithelial cells from corneal to conjunctival phenotype. The palisades of Vogt were defined as radial hyperreflective stromal ridges that follow a branching or interconnecting pattern alternated with columns of limbal basal epithelium (rete pegs) [30, 34, 35].

Central cornea epithelial phenotype and limbal IVCM images were acquired before and 12 months after MSCT and CLET therapies. The IVCM images were obtained and later analyzed, always by the same experienced researcher (I.P.S.) using the Heidelberg Eye Explorer software (V. 1.5.10.0. 2006; Heidelberg GmbH) to avoid interobserver variability. The main outcomes of the IVCM analysis were the epithelial phenotype of the central cornea (corneal, conjunctival, or mixed), and the presence or absence of transition zones and palisades of Vogt in the four quadrants of the limbus.

Statistical analysis was performed using R statistical package version 4.0.0. Quantitative characteristics were expressed as mean ± standard deviation (SD), and qualitative variables were described as numbers and percentages. McNemar's test was used to assess changes in the dichotomous variables before and 12 months after transplantation surgery, while Wilcoxon test was used for ordinal variables. To assess if there were any relationships between the changes in the epithelial phenotype of the central cornea after surgery and the changes in the palisades of Vogt and transition zones of the limbus, Mann–Whitney test was used.

Before surgery, 15 (eight MSCT and seven CLET) and eight (six MSCT and two CLET) LSCD eyes showed conjunctival and mixed epithelial phenotype for the central cornea, respectively. Twelve months after surgery, a conjunctival, mixed, and corneal epithelial phenotype was observed in eight (five MSCT and three CLET), five (two MSCT and three CLET), and ten (seven MSCT and three CLET) LSCD eyes, respectively. The improvement of the central corneal epithelial phenotype was significant not only for the whole sample (p < 0.001), but also for both the MSCT (p = 0.015) and the CLET (p = 0.026) groups.

Transition areas between corneal and conjunctival epithelium in any of the four quadrants of the limbus were found in nine (five MSCT and four CLET) LSCD eyes before surgery and in 16 (nine MSCT and seven CLET) LSCD eyes 12 months after cell transplantation. This change was only statistically significant (p = 0.046) for the nasal quadrant considering the total sample (Fig. 1), however, both MSCT (p = 0.31) and CLET (p = 0.08) groups independently did not show significant changes. Besides, there was not a significant association between the improvement in the epithelial phenotype of the central cornea and the higher number of transition zones observed (p ≥ 0.43).

Regarding the palisades of Vogt, they were found in any of the limbal quadrants in four (two MSCT and two CLET) LSCD eyes before surgery, and it increased to six (three MSCT and three CLET) LSCD eyes 12 months after surgery. This minor change was only significant in the inferior quadrant (p = 0.046) for the whole sample (Fig. 2). However, changes in the MSCT and CLET group were not significant (p = 0.08 and p = 0.31, respectively). There was not a significant (p ≥ 0.15) relationship between the improvement in the epithelial phenotype of the central cornea and the changes in the detection of palisades of Vogt. Representative cases of successful MSCT and CLET cases are shown in Figs. 3 and 4. Unsuccessful representative cases, in terms of absence of improvement in the limbus, are also shown in Fig. 1S and 2S (Supplementary material).