Evaluation of posterior capsule opacification of the Alcon Clareon IOL vs the Alcon Acrysof IOL using a human capsular bag model

Posterior capsule opacification (PCO) develops regularly after cataract surgery [1]. This unwanted wound healing reaction is thought to originate from lens epithelial cells that remain in the capsular bag after cataract surgery, especially on the inside of the anterior capsule and the capsular equator. After getting activated by several surgically and implant induced cytokines and growth-factors, cells undergo epithelial–mesenchymal transition to become myofibroblasts [2]. Those myofibroblasts proliferate and migrate on the posterior capsule towards the optical axis below the intraocular lens (IOL). Strong differentiation causes Elschnig pearls and Soemmering ring formations [3]. The condition results in increased light scattering and aberrations. Clinically, the patient is disturbed by reduced vision and increased straylight.

Recently the Clareon IOL (Alcon, Fort Worth, Texas, USA) was introduced. Its’ design is similar to the AcrySof IQ (Alcon, Fort Worth, Texas, USA), but the new material is made of a proprietary cross-linked acrylic optic biomaterial developed by combining a hydrophilic polymer (2-hydroxyethyl-methacrylate) and a hydrophobic component (phenylethyl acrylate) with a chemically bonded ultraviolet blocker, a blue-light filtering chromophore and a water content of 1.5%, which is supposed to show reduced glistening and surface inhomogeneities [4]. The producing company also claims a new precision edge design to be possible with this material, featuring a modified posterior square optic edge to minimize positive dysphotopsias and prevent PCO [5]. The AcrySof single-piece IOL has been introduced about 20 years ago, showing PCO with a consecutive Nd:YAG laser capsulotomy rate of slightly above 10% after 10 years of implantation [5]. The IOL has a sharp optic edge, which is interrupted at the haptic optic junction and is made of a hydrophobic acrylic polymer mix (phenylethyl methacrylate, phenylethyl acrylate, butanediol diacrylate) [6].

Both, the IOL material [7] and the edge design, play a critical role in PCO formation and rate [8]. The IOL materials’ influence is supposedly due to the different binding properties of extracellular matrix proteins like fibronectin and vitronectin, which promote cell growth [9]. With respect to PCO-preventive IOL design efforts, the sharp edge is intended to act as a mechanical barrier for lens epithelial cells. In this instance, the capsule is shrinking through peripheral fibrosis and wrapped tightly across the sharp edge [10]. The AcrySof IQ and the Clareon are different in IOL material and square edge design, with potential improvements towards the newly developed Clareon IOL.

The aim of this study was to compare the timing of ex-vivo PCO formation after implantation of the Clareon in comparison with the AcrySof IOL. PCO develops over several years, with incidence numbers increasing up to 9 years after implantation of the IOL [11]. As the Clareon is a newly introduced IOL, there is little data on long-term incidence. To obtain an early assessment of PCO formation, the human capsular bag model is commonly used [12, 13] to accelerate PCO formation ex vivo. Minor differences in PCO formation after implanting an IOL can be observed to test new IOL designs and types [14‐16]. Posterior capsule opacification as a type of fibrosis cannot only be reduced to cellular growth. Several molecular changes in the lens epithelial cells are observed [2]. Therefore and to obtain a valid comparison between the two IOL designs different molecular markers for fibrosis have been stained.

The new Clareon-IOL was developed with a precision sharp edge and a purported improvement in IOL material. Both, IOL material [18] and the square edge design [10], play a critical role in PCO formation. In our ex vivo study, we could not determine any differences in PCO formation of the newer Clareon when compared to the AcrySof IOL. Furthermore, there was a comparable fibrotic response regarding different molecular markers of fibrosis, which is in line with other reports [5]. In a recent meta-analysis of the AcrySof single and multi-piece models, data of three Alcon internal clinical trials on PCO formation of the Clareon were included [5]. Both the Clareon single-piece and multi-piece IOLs were investigated. Even though exact data of the trials are not presented, there were comparable results between the Clareon and the AcrySof Nd:YAG probability at 1 and 3 years, whereas only one of the three studies had three-year results. The authors concluded that the Clareon is likely to perform as well as, and possibly better than, AcrySof in terms of Nd:YAG capsulotomy rates. Furthermore, an in vivo rabbit study in fifteen New Zealand white rabbits with a follow up of 1 month did not detect a difference in PCO and anterior capsule opacification, as observed during clinical and pathological evaluation between the Clareon and the AcrySof IOL [19]. Our human ex vivo data in the capsular bag model shows a comparable result.

In comparison to other currently available IOL models, the AcrySof model has shown a low incidence of PCO in many thousand eyes in several population based studies and meta-analyses [5, 20]. Our study and other aforementioned, previous studies have shown a comparable performance of the Clareon and the AcrySof. This might be due to the precision edge of Clareon, which features a square posterior optic edge similar to that of the AcrySof. Even though the results show comparable PCO rates, the manufacturer claims potential advantages of the Clareon regarding less glistening, less axial displacement and reduced dysphotopsias and glare.

Myofibroblastic cells are a hallmark of PCO formation. Epithelial mesenchymal transformation of lens epithelial cells [21] or a direct, myogenic cell precursor called the Myo/Nog cells, are thought to be the origin of those myofibroblasts [22]. Several growths factors and cytokines can cause their activation, leading to cell growth, migration, fibrosis and contraction of the posterior capsule [3]. In order to be able to cause this unwanted wound healing reaction, cells have to express certain proteins and cellular behavior, which are not present in healthy lens epithelial cells. α-SMA is one of the proteins involved in contraction of cells and is usually present in human explanted post-mortem capsular bags with PCO [23] and implicated in PCO formation [24]. In our experiments, we detected an equal amount of α-SMA positive cells in the groups with IOL implantation and cell presence was enhanced in empty capsular bags without IOL. Hence, the implantation of an IOL seems to block the formation of epithelial-mesenchymal transition of cells at the posterior lens capsule. Collagen type 1 is a secreted protein and produced by lens epithelial cells when undergoing fibrotic reactions [25] and is therefore also a marker for myofibroblastic activity. Collagen type 1 was visible extracellular and on top of the posterior capsule and especially in the capsular folds seen in the group without IOL. To our knowledge collagen type 1 is not found in the healthy capsule [26], yet previous post-mortem human studies have shown that it is highly abundant in the fibrous extracellular matrix typically found in PCO (e.g. Elschnig pearls and Soemmering ring) [27]. Furthermore, it can accelerate fibrosis by direct interaction with lens epithelial cells through metallo-matrix proteinases in lens epithelial cells [28]. This might explain why its presence is higher in the capsular folds, where fibrosis is increased. Myofibroblasts furthermore overexpress fibronectin, which allows them to bind to extracellular matrix. Fibronectin modulates and stabilizes the extracellular matrix in wound healing processes [29]. Fibronectin was present in the expected location extracellularly and enhanced below the IOLs and in the capsular folds, where increased fibrotic cell activity is suspected [21].

Limitations of this study include the experimental laboratory character and the use of fetal calf serum (FCS). The human capsular bag cells do still actively synthesize proteins and growth factors which accelerates their growth following more than 1 year in protein-free medium in cell culture [30]. The finding that persistent cell proliferation can occur is significant, as it suggests that lens epithelial cells have a baseline ability to remain active and contribute to PCO development, which typically becomes clinically relevant years after surgery [31]. Due to a many month-long incubation of the capsular bags being out of scope for this study, we added FCS, which contains various growth factors, to accelerate epithelial mesenchymal transition and proliferation of the cells. The scientific community is currently still in discourse on what is the appropriate amount of FCS for the capsular bag growth model. The used percentage varies widely from 0 to 10% across the literature and depends on the scientific requirements and the hypothesis [12, 30]. The higher the concentration of FCS, the faster the PCO formation. In contrast, individual factors like donor age contributing to PCO formation are less relevant to the present analysis, since only donor pairs of eyes were used to compare PCO formation between both IOLs. After careful consideration we choose 3% FCS as it is still high enough to allow individual donor factors which seems more clinically relevant.

Our study clearly demonstrates that the new Clareon IOL shows no difference in terms of PCO formation when compared to the AcrySof IOL in the human ex vivo capsular bag model. Cellular growth was comparable, and all tested fibrotic markers did not vary between the two IOLs. Both IOLs had a protective effect on PCO development after implantation when compared to capsular bags without IOL implantation.