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Editors Selection IGR 15-1

Anatomical Structures: Distal Aqueous Outflow Pathways

Nils Loewen
Choa Wang

Comment by Nils Loewen & Choa Wang on:

75468 Deep tissue analysis of distal aqueous drainage structures and contractile features, Gonzalez JM; Ko MK; Hong YK et al., Scientific reports, 2017; 7: 17071


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Gonzalez et al.1 present a smorgasbord of images of the distal outflow tract of the mouse in a total of 14 figures with up to 20 subpanels per figure. The authors had several goals that were rather ambitious: (1) to establish 2-photon deep tissue imaging with 3D reconstruction of the imaging data; (2) to distinguish blood from lymphatic markers; and (3) to detect structures suggesting contractility. The primary technique applied in these studies has a name that is almost as long as the list of goals: 'trans-scleral multimodal 2-photon imaging with 2-photon excitation fluorescence and second harmonic generation (2P TPEF SHG)'. 2P TPEF SHG uses deep red and near infrared light to penetrate tissue deeper than visible light used in standard confocal microscopy. It has reduced scattering which allows the fluorescent target to be well identified. The principal behind 2P TPEF SHG is that when two photons with the same frequency interact with a non-linear material they are combined in a process called second harmonic generation which generates a new photon with twice the energy of the initial photons. The difference between the exciting and the emitting light allows for easy separation of the second harmonic generation signal and a high axial and lateral resolution that is comparable to that of confocal microscopy but without having to use pinholes.

This technique is impressive and useful because it allows imaging tissues in vivo up to 100 to 200 microns2 with a resolution that allows to distinguished structures several microns in size. The practically achievable depth depends on the amount of light scatter, however. A downside of 2P TPEF SHG is that fluorophores are necessary which requires either the use of transgenic animals with fluorescent proteins or ex vivo stains or antibodies. In contrast to confocal microscopy, that can achieve up to 365 nm resolution at 2 mm depth,3,4 the tissue does not have to be made transparent.

If a bit overwhelming at first, Gonzalez et al.'s manuscript is a treasure trove for outflow researchers that convincingly demonstrates that features are present in the distal outflow tract of the mouse that should allow it to actively contract and dilate. Recent studies show that the distal outflow tract can indeed regulate outflow and IOP by contracting and dilating in human and porcine eyes.5,6 Interestingly, the distal outflow tract endothelium was Prox1-positive, CD31-positive but LYVE-1-negative, giving it a signature different from blood and true lymphatic vessels. Schlemm's canal is a VEGF-C/VEGFR3-responsive lymphatic-like vessel7 that develops from transscleral veins8 and emerges together with the collector channels. While disappointing that not more lymphatic features were seen in the distal outflow tract of the mouse, they may play a more prominent role in larger primate eyes. Lymphatic features in direct proximity to these structures are already known to get activated by epibulbar glaucoma surgery where aqueous is shunted into an artificial conjunctival fluid pocket and absorbed by lymphatics.8 Recent discoveries on prostaglandin analogs, arguably the most successful eye drops in glaucoma, showed that in addition to enhancing uveoscleral outflow, they increase contraction and propulsion of lymphatics.9

References

  1. Tan JC, Gonzalez J, Ko MK, Masedunskas A, Weigert R, Hong Y. Contractile features of the distal aqueous drainage tract. Invest Ophthalmol Vis Sci. 2017;58(8):3771-3771.
  2. Durr NJ, Weisspfennig CT, Holfeld BA, Ben-Yakar A. Maximum imaging depth of two-photon autofluorescence microscopy in epithelial tissues. J Biomed Opt. 2011;16(2):026008.
  3. Waxman S, Loewen RT, Dang Y, Watkins SC, Watson AM, Loewen NA. High-resolution, threedimensional reconstruction of the outflow tract demonstrates segmental differences in cleared eyes. Invest Ophthalmol Vis Sci. 2018;59(6):2371-2380.
  4. Watson AM, Rose AH, Gibson GA, et al. Ribbon scanning confocal for high-speed highresolution volume imaging of brain. PLoS One. 2017;12(7):e0180486.
  5. McDonnell F, Dismuke WM, Overby DR, Stamer WD. Pharmacological regulation of outflow resistance distal to Schlemm's canal. Am J Physiol Cell Physiol. April 2018. doi:10.1152/ ajpcell.00024.2018
  6. Waxman S, Wang C, Dang Y, et al. Structure-function changes of the distal outflow tract in response to nitric oxide. Preprint. May 2018. doi:10.20944/preprints201806.0075.v1
  7. Aspelund A, Tammela T, Antila S, et al. The Schlemm's canal is a VEGF-C/VEGFR-3- responsive lymphatic-like vessel. J Clin Invest. 2014;124(9):3975-3986.
  8. Yu D-Y, Morgan WH, Sun X, et al. The critical role of the conjunctiva in glaucoma filtration surgery. Prog Retin Eye Res. 2009;28(5):303-328.
  9. Tam ALC, Gupta N, Zhang Z, Yücel YH. Latanoprost stimulates ocular lymphatic drainage: An in vivo nanotracer study. Transl Vis Sci Technol. 2013;2(5):3.

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