The effect of eye fixation on IOP during the FLACS procedure is a concern as shown by previous studies.
5,6,9 Table 2 provides a summary of published studies regarding IOP during FLACS procedures. Talamo et al.
6 conducted invasive IOP measurements in cadaver eyes by comparing an applanating corneal interface to the LOI, which was also the approach used in the present study. The measurements by Talamo et al.
6 were performed only during the first step of the Catalys docking procedure (vacuum). IOP elevation at this point was reported as 16.6 mm Hg ± 1.8 SD. These results are similar to our findings during the initial stage of the femtosecond laser docking procedure. It should, however, be noted that Talamo et al. did not set the cadaver eyes to a constant starting IOP. Furthermore, they did not fully connect the cadaver eyes to the laser system and no laser treatment was performed.
Ibarz et al.
10 started their experiments at very low IOP levels (5.67 mm Hg ± 2.39). As the ocular pressure–volume relationship is an exponential function, this makes a direct comparison of the results difficult; that is, if different eyes are measured with different baseline IOP levels, the same volume displacement will yield very different pressure values.
Schultz et al.
8 and Kerr et al.
9 evaluated IOP elevations in patients undergoing a Catalys femtosecond laser procedure performed using noninvasive applanating methods. Schultz et al.
8 reported a mean IOP elevation to 27.7 mm Hg ± 5.5 SD after a femtosecond laser procedure conducted using a customized Schiotz Tonometer. Using an iCarePRO Tonometer (Tiolat, Oy, Finland), Kerr et al.
9 also observed IOP elevations to 36.0 ± 4.4 mm Hg after femtosecond laser treatment. Both groups were able to record IOP elevations with the LOI connected to the eye, but not during the complete femtosecond laser treatment. Furthermore, changes in the corneal surface tension caused by the LOI when the vacuum is applied may influence the values obtained from an indention/rebound measurement method.
Using a Tono-Pen Avia (Reichert Technologies, Depew, NY, USA), Baig et al.
11 utilized a different femtosecond cataract laser platform with a multipiece curved interface to also perform IOP measurements on humans. Mean IOP was reported to rise to 42.1 ± 10.8 mm Hg after the femtosecond procedure. These discrepancies across studies suggest that rises in IOP vary with different femtosecond cataract laser systems. Interestingly, all the in vivo studies reported IOP elevations after femtosecond laser treatment, whereas we did not find any such elevations in the experimental setup of the present study after the eye was fully disconnected from the LOI.
6,8,9,11
There are probably different causes of the IOP increases during the different steps of the FLACS procedure. As shown in
Figures 2 and
3, a significant change occurs immediately after placing the patient interface on the enucleated eye. The IOP elevations during the connecting procedure are caused by the volume displacement by the weight of the laser lens and the applied force. More interestingly, the IOP rises significantly during lens fragmentation, with the most likely cause being the gas formation that occurs at this point, as this correlates with the tissue fragmentation time and, thereby, the volume (
Fig. 4).
When using cadaver eyes for IOP measurements, the shortcomings of the experiment must be noted. The influence of the ocular blood volume of the living eye on the pressure–volume relationship cannot be simulated. This interpretation is supported by previous investigations showing differences in ocular rigidity before and after enucleation.
12,13 Figure 5 shows the course of the IOP in the eye of a living rabbit in response to the continuous infusion of a balanced salt solution into the vitreous cavity. The graph shows the marked differences between the IOP response predicted by the Friedenwald equation and the IOP response in a living eye.
\(\def\upalpha{\unicode[Times]{x3B1}}\)\(\def\upbeta{\unicode[Times]{x3B2}}\)\(\def\upgamma{\unicode[Times]{x3B3}}\)\(\def\updelta{\unicode[Times]{x3B4}}\)\(\def\upvarepsilon{\unicode[Times]{x3B5}}\)\(\def\upzeta{\unicode[Times]{x3B6}}\)\(\def\upeta{\unicode[Times]{x3B7}}\)\(\def\uptheta{\unicode[Times]{x3B8}}\)\(\def\upiota{\unicode[Times]{x3B9}}\)\(\def\upkappa{\unicode[Times]{x3BA}}\)\(\def\uplambda{\unicode[Times]{x3BB}}\)\(\def\upmu{\unicode[Times]{x3BC}}\)\(\def\upnu{\unicode[Times]{x3BD}}\)\(\def\upxi{\unicode[Times]{x3BE}}\)\(\def\upomicron{\unicode[Times]{x3BF}}\)\(\def\uppi{\unicode[Times]{x3C0}}\)\(\def\uprho{\unicode[Times]{x3C1}}\)\(\def\upsigma{\unicode[Times]{x3C3}}\)\(\def\uptau{\unicode[Times]{x3C4}}\)\(\def\upupsilon{\unicode[Times]{x3C5}}\)\(\def\upphi{\unicode[Times]{x3C6}}\)\(\def\upchi{\unicode[Times]{x3C7}}\)\(\def\uppsy{\unicode[Times]{x3C8}}\)\(\def\upomega{\unicode[Times]{x3C9}}\)\(\def\bialpha{\boldsymbol{\alpha}}\)\(\def\bibeta{\boldsymbol{\beta}}\)\(\def\bigamma{\boldsymbol{\gamma}}\)\(\def\bidelta{\boldsymbol{\delta}}\)\(\def\bivarepsilon{\boldsymbol{\varepsilon}}\)\(\def\bizeta{\boldsymbol{\zeta}}\)\(\def\bieta{\boldsymbol{\eta}}\)\(\def\bitheta{\boldsymbol{\theta}}\)\(\def\biiota{\boldsymbol{\iota}}\)\(\def\bikappa{\boldsymbol{\kappa}}\)\(\def\bilambda{\boldsymbol{\lambda}}\)\(\def\bimu{\boldsymbol{\mu}}\)\(\def\binu{\boldsymbol{\nu}}\)\(\def\bixi{\boldsymbol{\xi}}\)\(\def\biomicron{\boldsymbol{\micron}}\)\(\def\bipi{\boldsymbol{\pi}}\)\(\def\birho{\boldsymbol{\rho}}\)\(\def\bisigma{\boldsymbol{\sigma}}\)\(\def\bitau{\boldsymbol{\tau}}\)\(\def\biupsilon{\boldsymbol{\upsilon}}\)\(\def\biphi{\boldsymbol{\phi}}\)\(\def\bichi{\boldsymbol{\chi}}\)\(\def\bipsy{\boldsymbol{\psy}}\)\(\def\biomega{\boldsymbol{\omega}}\)\(\def\bupalpha{\unicode[Times]{x1D6C2}}\)\(\def\bupbeta{\unicode[Times]{x1D6C3}}\)\(\def\bupgamma{\unicode[Times]{x1D6C4}}\)\(\def\bupdelta{\unicode[Times]{x1D6C5}}\)\(\def\bupepsilon{\unicode[Times]{x1D6C6}}\)\(\def\bupvarepsilon{\unicode[Times]{x1D6DC}}\)\(\def\bupzeta{\unicode[Times]{x1D6C7}}\)\(\def\bupeta{\unicode[Times]{x1D6C8}}\)\(\def\buptheta{\unicode[Times]{x1D6C9}}\)\(\def\bupiota{\unicode[Times]{x1D6CA}}\)\(\def\bupkappa{\unicode[Times]{x1D6CB}}\)\(\def\buplambda{\unicode[Times]{x1D6CC}}\)\(\def\bupmu{\unicode[Times]{x1D6CD}}\)\(\def\bupnu{\unicode[Times]{x1D6CE}}\)\(\def\bupxi{\unicode[Times]{x1D6CF}}\)\(\def\bupomicron{\unicode[Times]{x1D6D0}}\)\(\def\buppi{\unicode[Times]{x1D6D1}}\)\(\def\buprho{\unicode[Times]{x1D6D2}}\)\(\def\bupsigma{\unicode[Times]{x1D6D4}}\)\(\def\buptau{\unicode[Times]{x1D6D5}}\)\(\def\bupupsilon{\unicode[Times]{x1D6D6}}\)\(\def\bupphi{\unicode[Times]{x1D6D7}}\)\(\def\bupchi{\unicode[Times]{x1D6D8}}\)\(\def\buppsy{\unicode[Times]{x1D6D9}}\)\(\def\bupomega{\unicode[Times]{x1D6DA}}\)\(\def\bupvartheta{\unicode[Times]{x1D6DD}}\)\(\def\bGamma{\bf{\Gamma}}\)\(\def\bDelta{\bf{\Delta}}\)\(\def\bTheta{\bf{\Theta}}\)\(\def\bLambda{\bf{\Lambda}}\)\(\def\bXi{\bf{\Xi}}\)\(\def\bPi{\bf{\Pi}}\)\(\def\bSigma{\bf{\Sigma}}\)\(\def\bUpsilon{\bf{\Upsilon}}\)\(\def\bPhi{\bf{\Phi}}\)\(\def\bPsi{\bf{\Psi}}\)\(\def\bOmega{\bf{\Omega}}\)\(\def\iGamma{\unicode[Times]{x1D6E4}}\)\(\def\iDelta{\unicode[Times]{x1D6E5}}\)\(\def\iTheta{\unicode[Times]{x1D6E9}}\)\(\def\iLambda{\unicode[Times]{x1D6EC}}\)\(\def\iXi{\unicode[Times]{x1D6EF}}\)\(\def\iPi{\unicode[Times]{x1D6F1}}\)\(\def\iSigma{\unicode[Times]{x1D6F4}}\)\(\def\iUpsilon{\unicode[Times]{x1D6F6}}\)\(\def\iPhi{\unicode[Times]{x1D6F7}}\)\(\def\iPsi{\unicode[Times]{x1D6F9}}\)\(\def\iOmega{\unicode[Times]{x1D6FA}}\)\(\def\biGamma{\unicode[Times]{x1D71E}}\)\(\def\biDelta{\unicode[Times]{x1D71F}}\)\(\def\biTheta{\unicode[Times]{x1D723}}\)\(\def\biLambda{\unicode[Times]{x1D726}}\)\(\def\biXi{\unicode[Times]{x1D729}}\)\(\def\biPi{\unicode[Times]{x1D72B}}\)\(\def\biSigma{\unicode[Times]{x1D72E}}\)\(\def\biUpsilon{\unicode[Times]{x1D730}}\)\(\def\biPhi{\unicode[Times]{x1D731}}\)\(\def\biPsi{\unicode[Times]{x1D733}}\)\(\def\biOmega{\unicode[Times]{x1D734}}\)\begin{equation}{\rm{IO}}{{\rm{P}}_{\rm{2}}} = {\rm{\ 1}}{0^{(k*{\rm{dV}} + {\rm{log\,IOP_1}})}}\end{equation}
where IOP = intraocular pressure,
k = rigidity factor, dV = volume increment.
The Friedenwald equation describes the pressure–volume relationship in relation to the rigidity of the eye (rigidity factor
k). The higher this rigidity, the higher the increase in IOP in response to a particular ocular volume change. Given that the pressure–volume relationship is different in perfused and enucleated eyes, pressure–volume relationships from the literature can be used to estimate the in vivo IOP during the femtosecond laser procedure.
12,14 In our study, we observed peak IOP levels of 54 mm Hg during fragmentation. The Friedenwald equation allows a theoretical calculation of the IOP increases that can be expected in a perfused eye, based on the assumption that the choroidal blood volume acts as a buffer for IOP changes. An IOP of 54 mm Hg equates to a volume increase of 50 μL. The choroidal blood volume is assumed to be approximately 250 μL. Therefore, a calculated volume increase of 50 μL will lead to only a moderate increase of IOP in a living eye, as it can be buffered by the choroidal volume.
In addition, it is possible to estimate the forces on the lens capsule during the laser lens fragmentation.
Figure 2 shows the IOP trace during the femtolaser treatment. We can deduce from the IOP changes between the beginning and end of lens fragmentation that an IOP elevation of 5 mm Hg occurs during this process. Following the Friedenwald equation, this IOP elevation is caused by a volume increase of 2.5 μL. This increase occurs from the gas formation during lens fragmentation. According to the literature, an elevation of 2.5 μL leads to a intracapsular pressure elevation of less than 10 mm Hg.
15 This elevation of intracapsular pressure is of special interest, because it might lead to tears or even ruptures of the lens capsule during femtosecond laser treatment. The porcine lens volume is approximately 400 μL.
16 This means that the lens capsule has to resist an intracapsular volume increase of 0.625%. Biomechanical studies on porcine lens capsules show a much higher resistance to strain and stress until the capsule fails compared to human lens capsules.
17 Assuming that a similar intracapsular pressure elevation is created during femtosecond laser treatment of a human lens, and applying the findings of Fischer
15 in terms of the strength of the human lens capsule, the gas volumes generated in our experiments do not pose a threat to human lens capsule integrity during femtosecond laser cataract treatment. Additionally, it should be noted that lens fragmentation is followed by capsulotomy, and so the produced gas has space to escape the intracapsular compartment.
On the other hand, we need to consider that our experiments were performed on clear porcine lenses and so less laser energy was needed for lens fragmentation. In humans, gas formation during laser lens fragmentation could reach higher levels, because more laser energy is needed to treat opaque lenses. This assumption is supported by the higher IOP values after femtosecond laser treatment on humans reported by other groups.
8,9
In conclusion, significant IOP elevations occur during the FLACS procedure, as shown by our findings and data from previous studies. The discrepancies of our findings compared to previous literature may be explained by the different study designs.