Identifying protease-resistant domains in the bead region

The binding sites of two monoclonal antibodies (mAbs) raised against the N-terminal half of fibrillin have previously been mapped on the microfibril structure^13,38. mAb1919 binds within the arm region, whereas mAb2502 binds on the side of the bead and specifically recognizes human microfibrils. Using short recombinant human fibrillin constructs¹⁹, we narrowed down the antibody-binding sites by western blotting (Extended Data Fig. 2a,b). The epitope for mAb2502 was refined considerably as it detected two overlapping fibrillin constructs that restricted the epitope to within domains TB1 and the PRR. mAb1919 detected a construct containing domains cbEGF7–hybrid2 immediately downstream of TB2 (Extended Data Fig. ​Fig.2b).2b). Taken together, these data suggest that TB1 and/or the PRR are located on the peripheral edge of the bead, whereas domains downstream of TB2 are found in the arm/interbead region. Our recent mass spectrometry data identified a protease-resistant fibrillin region comprizing domains EGF4–TB2 (ref. ⁴¹). Peptides from this region were never detected by liquid chromatography with tandem mass spectrometry after elastase digestion of microfibrils from skin, fibroblast cultures or ciliary body (Extended Data Fig. ​Fig.2c).2c). These findings are consistent with other proteomics studies on microfibrils from ciliary zonules digested with trypsin, where few peptides from this region were identified^42,43. Taking this into account, together with the antibody epitope mapping data, we suggest that the EGF4–TB2 domains could be buried in the bead core and thus protected from proteolytic digestion (Extended Data Fig. ​Fig.2d2d).

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Extended Data Fig. 2

Refining epitope labelling of fibrillin recombinant fragment.

Mab2502 (clone 26 (epitope within residues 45–450 from epitope mapping¹³)) and Mab1919 (clone 11C1.3 (epitope within residues 451–909 as defined by manufacturer)) were used to probe overlapping recombinant fibrillin fragments to more accurately define their epitopes in fibrillin-1. (Ai and Bi) schematic diagrams of recombinant fragments N-Ter, PF1, PF2, PF3, PF4, PF5, Ex3-11 and Ex4-11. Recombinant fibrillin-1 fragments after separation by SDS-PAGE in the presence (R) or absence (NR) of a reducing agent followed by western blotting with either (Aii) Mab2502 or (Bii) Mab1919. These blots were repeated at least 3 times. The antibody epitopes for mab2502 (45–450¹³) and mab1919 (451–909) are narrowed down to TB1-PRR (residues 330–450) and cbEGF7-Hyb2 (residues 723-909) respectively, highlighted in red. (C) Number of peptides identified by LC-MS/MS from each domain of fibrillin, where a protease resistant region is located between TB1 to TB2 (TB domains are numbered) and indicated by an asterisk (redrawn from⁴¹). (D) Diagram of the fibrillin microfibril repeating unit with the binding sites of Mab2502 and Mab1919 in adult human ciliary zonule microfibrils (as determined in³⁸) and putative location of the protease resistant region identified in⁴¹. Panel c adapted from ref. ⁴¹ under a Creative Commons licence CC BY 4.0.

Modeling the terminal regions into the fibrillin bead

The cryo-EM reconstruction was analyzed for regions that were buried in the core of the interwoven bead structure. A feature was observed in the center of the bead map that remained connected at high threshold levels (Fig. ​(Fig.2a).2a). This feature could be traced through the center of the bead and was found to have a persistence length of 17nm (measured with UCSF Chimera using volume tracer), where a diameter of ~2nm was consistent with the width of the EGF and TB domains and the length supported a chain of around seven domains. Within the bead, there are four nonsymmetric copies of this chain (Fig. ​(Fig.2b),2b), which appear twice due to the twofold symmetry, confirming the previously seen pseudo eightfold symmetric arrangement of eight fibrillin monomers per repeat within the fibrillin microfibril^37,44. Three of these features are of similar dimensions but the fourth is shorter. This may be due to loss of density in the averaging caused by the flexibility of the arms. Moreover, the arm region was not under the 3D mask during refinement of the bead. The interface between the bead and arm could be seen more clearly in a lower-resolution reconstruction in which a larger mask was used for refinement (Extended Data Fig. ​Fig.3).3). Guided by the antibody mapping data and starting at the edge of the bead, domain TB1, followed by the consecutive domains from PRR to cbEGF6, is docked into the density for one of these regions. The density where domains cbEGF5 and cbEGF6 are docked is contiguous with the density for the arm regions, giving confidence to these domain assignments. A small-angle X-ray scattering (SAXS)-derived model of this region was used to aid this docking (Fig. 2c (i)). The arrangement of these domains in the cryo-EM structure is very similar to the model based on experimental SAXS data⁴⁵.

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Fig. 2

Modeling of the fibrillin N-terminal region into the fibrillin bead region.

a, Cryo-EM structure of the fibrillin bead region with a feature (in the centre of the bead map) that remained connected at high threshold levels segmented and highlighted in blue. b, The four unique (not symmetry-related) copies of this region are segmented from the bead map. The feature shown in a is colored blue. As twofold symmetry has been applied to the reconstruction, there are also symmetric pairs of each of these features to give eight in total in the bead core. c, (i) A SAXS-derived model of the region encompassing TB1, the PRR, EGF4 and cbEGF3–6 (ref. ⁴⁵) is docked into the region from the core of the bead segmented in a (shown as pale blue density). (ii) A cross-section through the bead density is shown with schematic representation of the N-terminal region (blue) running through the core of the bead (as modeled in c (i)) and C-terminal region (red) in the outer density. On the right, an alternative representation is presented where the C-terminal region could be in the inner core of the bead with the N-terminal region around the outside. In both, the cbEGF5 and cbEGF6 domains would be in the same location as their connection to the density in the arm region is contiguous. d, The four central densities shown in b and their symmetric pairs are segmented from the bead structure and colored as in b and are shown without the remaining bead structure. e, As in d, but shown with the remaining bead density colored gray.

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Extended Data Fig. 3

Fibrillin arm region reconstruction.

a) 3D reconstruction of the bead region shown in three orthogonal orientations. There are 8 arms which are visible emerging from the bead structure. Highlighted with black arrows are two arms which are wider. The red arrows highlight two arm regions which are masked out in the final bead reconstruction. b) The reconstruction in (A) is shown overlaid on the final bead reconstruction shown in grey. Panel (Bii) shows a magnified view of the arm regions connecting to the bead region. The red arrow shows how the wider arms connects to the outside of the bead, in contrast the arm highlighted by the black arrow inserts into the centre of the bead.

Due to the dense molecular packing in the bead region and lower local resolution in the bead core region (Extended Data Fig. ​Fig.1d),1d), it is possible that the molecules in the core of the bead take a different path through the center of the bead. Antibody binding data have previously shown that the C-terminal region of fibrillin is also located near to the bead^13,38 and the C-terminal half of fibrillin-1 has been shown to self-assemble into bead-like multimers that have been suggested to initiate microfibril assembly¹⁶. Furthermore, there are differences in the predicted location of the N-terminal region in microfibrils purified from adult human ciliary zonule and human neonate foreskin, suggesting that the mab2502 (clone 26) epitope may be conformationally variable^13,38. Therefore, we modeled an alternative path through the bead core, where the central core may be composed of N- and C-terminal interacting regions (Fig. 2c (ii)), consistent with antibody mapping data. Importantly, domains cbEGF5 and cbEGF6 would remain in the same location in both scenarios, as these domains connect and are contiguous with the density that continues into the arm region.

After accounting for the eight copies of this central region within the core of the microfibril bead (Fig. ​(Fig.2d),2d), the remaining bead structure forms a ring around the outside surface and interwoven on the underside of the bead, as shown in gray in Fig. ​Fig.2e.2e. The approximate mass of the bead region estimated from the cryo-EM electron density map is ~1.1MDa, which is consistent with STEM mass mapping. After docking eight symmetric copies of these seven fibrillin domains into the bead core, there is still sufficient mass and density to accommodate a further 12 or so fibrillin domains for each of the eight symmetric copies (supported by the eightfold pseudosymmetry). This suggests that there is quite an extensive overlap of N- and C-terminal regions within the bead.

Mutated microfibrils reveal a disrupted shoulder region

After locating the domains downstream of TB1 in the bead region, we predicted that the upstream N-terminal domains would be in the shoulder region. To confirm this, microfibrils from two fibrillin mouse models with either a domain deletion upstream, or downstream including the TB1 domain, were analyzed. Imaging these microfibrils allowed us to confirm the positions of these domains in the microfibril reconstruction and to analyze the structural consequences of deletion of fibrillin domains on microfibril structure. Microfibrils were purified from skin from 6-week-old mice homozygous for either a deletion of the first hybrid domain (ΔH1) (ref. ³⁵); a domain that contributes to the fibrillin-binding site for latent TGFβ via LTBP-1 (ref. ²⁷) or a deletion of three domains (TB1–PRR–EGF4) that causes WMS³⁶. As microfibrils are more difficult to extract from skin, negative staining electron microscopy was used to image microfibrils, as it has a much higher signal-to-noise ratio than cryo-EM and can gain more information from fewer microfibrils. A total of 100 microfibril periods were measured for each dataset and compared with wild-type microfibrils (Fig. 3a,b). The control microfibrils had a periodicity of 57.95±0.22nm. The ΔH1 microfibrils had a periodicity of 57.14±0.27nm, which was 0.81nm shorter than that of the control. The WMS microfibrils had a periodicity of 55.21±0.26nm, which was 2.75nm shorter than that of the control. These data show that although microfibrils are formed with their main features preserved, the deletion of either one or three domains decreases microfibril periodicity proportionally.

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Fig. 3

Mutant fibrillin microfibrils reveal a disrupted shoulder region.

Fibrillin microfibrils extracted from control and homozygous WMS and H1 mouse skin and imaged using negative stain TEM. a, Representative TEM images of (i) control, (ii) WMS and (iii) H1 extracted fibrillin microfibrils. Scale bars, 100 nm. Schematic of the fibrillin domain structure is shown above each image, with the WMS and ΔH1 domain deletions represented as dotted lines. b, Scatter plot showing the periodicities of the control, WMS and H1 extracted fibrillin microfibrils. The data represent means±s.d. For each dataset, 100 microfibril periods were measured and statistical analysis shows that the mutated microfibrils were significantly different from the control (*P=0.042; ****P<0.0001), as determined by one-way analysis of variance with Dunnett’s multiple comparisons test. c, Averaged images were generated from 458 wild-type periods, 472 H1 periods and 476 WMS periods. The top panels show 2D plots of the stain exclusion/intensity profile across the averaged fibrillin microfibril period (bottom panels) for (i) control, (ii) WMS and (iii) H1 microfibrils. The red arrows highlight a region at one side of the bead of the microfibril that is disrupted in the mutated microfibrils.

Source data

Averages from 458 wild-type periods, 472 H1 periods and 476 WMS periods of the microfibril repeating units were made and analyzed for changes in microfibril structure. In both cases for the mutants, structural features in the shoulder region are lost (Fig. ​(Fig.3c),3c), with the shoulder to the bead peak (seen in the control at ~35nm) being no longer distinct in WMS and ΔH1 microfibrils. This feature is immediately adjacent to the modeled location of the fibrillin domains through the bead (Fig. ​(Fig.2c).2c). These findings support the location of the TB1 domain in this region and the docking of these domains near the bead region. For both deletions, the perturbation spans a few nanometers, suggesting that the deletions may influence the conformation of neighboring domains.

LTBP-1 binding is perturbed by a WMS-causing mutation

Given the conformational disruption observed in the mutated microfibrils, we predicted that the WMS deletion of domains TB1–PRR–EGF4 could perturb the interaction of microfibril-binding proteins that bind near to this deletion. To test this, we analyzed the binding of LTBP-1. LTBP-1 is not an integral microfibril component but interacts with the N-terminal region of fibrillin via the hybrid1 domain and adjacent EGF domains^27,46. To test whether the structural rearrangements observed in the WMS microfibrils could impact on interactions with fibrillin-binding partners, we analyzed the binding of the LTBP-1 C-terminal region to a fibrillin construct containing the WMS deletion. Surface plasmon resonance showed that the affinity of LTBP-1 for fibrillin is decreased with the WMS deletion (Fig. 4a,b). The LTBP-1-binding epitope is two to four domains upstream of the domains deleted in WMS²⁷. This further supports longer-range structural rearrangements perturbing a binding site at least 50Å away when these domains are deleted.

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Fig. 4

LTBP-1 binds to the bead region of fibrillin microfibrils and is disrupted by a WMS-causing mutation.

a, SPR analysis of LTBP-1 binding to the N-terminal fragment PF3 of fibrillin with and without the WMS deletion. The LTBP-1 C-terminal region was immobilized to the sensor chip using amine coupling, and concentrations of PF3 (0–20nM) and PF3 WMS (0–50nM) were flowed over as analytes. Representative sensorgrams show the binding of PF3 or PF3 WMS to LTBP-1. This experiment was repeated three times. b, Binding kinetics, as determined using equilibrium analysis for the interaction of PF3 or PF3 WMS with LTBP-1. c, A complex of full-length LTBP-1 with purified fibrillin microfibrils was formed and analyzed using STEM mass mapping. (i) STEM images of fibrillin microfibrils with and without LTBP-1. Scale bars, 100nm. (ii) Scatter plot of the mass per microfibril repeat of fibrillin microfibrils (fib) with and without LTBP-1. The mean mass of a fibrillin repeat was 3,055±36.7kDa (n=75 from ten images). In complex with LTBP-1, the mass was 3,405±54.43kDa (n=69 from 11 images). The data represent means±s.d. Statistical significance was determined by unpaired two-tailed t-test (****P<0.0001). (iii) Trace of the mass per unit length (MUL) across the fibrillin repeat showing that there is a gain in mass at the bead region of the microfibril in the presence of LTBP-1. Each trace is an average of 50 periods (ten measurements from each of five images).

Source data

Furthermore, given the domain mapping (Fig. ​(Fig.2c)2c) and analysis of the ΔH1 microfibril structure (Fig. ​(Fig.3c),3c), we hypothesized that LTBP-1 would bind close to the bead region of the microfibril. LTBP-1 is not present (or is only present at very low abundance) in the ciliary zonules and so does not copurify with these microfibrils. Therefore, we bound full-length LTBP-1S to purified fibrillin microfibrils and looked for any increase in mass across the microfibril repeating unit using STEM mass mapping (Fig. ​(Fig.4c).4c). The microfibrils had a mean mass of ~3MDa per repeat, which is slightly larger than the mass expected for eight fibrillin molecules (~2.7MDa). This suggests that some microfibril-associated proteins (for example, MAGP1, which is typically present^42,43,47) might have been copurified. When LTBP-1S was added, there was an increase in mass across the microfibril repeat of 350.2±64.7kDa, which was localized predominantly to the bead region (Fig. ​(Fig.4c).4c). As the short splice form of LTBP-1 has a molecular weight of 151kDa, this increase in mass is consistent with two molecules of LTBP-1 binding per microfibril repeat.

Fibrillin arm region structure

The cryo-EM dataset from the fibrillin microfibrils was next recentered on the arm region and refined with a region-specific 3D mask. Particles that had been aligned to the full fibrillin repeat were recentered to locate the arm region coordinates at the particle center. After 3D classification, the resulting best class was refined using 3D auto-refine with C2 symmetry imposed down the fiber axis, as with the bead reconstruction. The structure of the fibrillin arm region showed eight arms that were continuous from the bead to the interbead region and two shorter densities (Fig. ​(Fig.5a).5a). Domains from TB2 to TB3 were docked into this region, guided by the domains located in the bead region and the antibody mapping of mAb1919 (which recognizes domains cbEGF7–hybrid2). Three distinct bands of higher density were observed in the 2D averages of microfibrils, correlating with the docked locations of domains TB2, hybrid2 and TB3, which have a larger mass than the EGF/cbEGF domains (Fig. ​(Fig.5c5c).

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Fig. 5

Fibrillin arm region structure.

The cryo-EM classes of the fibrillin microfibrils were recentered and refined to determine the structure of the fibrillin arm region. a, Cryo-EM structure of the arm region of fibrillin microfibrils. b, 2D class-averaged particles aligned to the fibrillin arm region reconstruction. Box size, 57nm. c, Domains docked into the arm region reconstruction from TB2 to TB3, where the larger TB and hybrid domains correspond to the densities observed in electron microscopy images.

Fibrillin microfibril extraction from bovine ciliary zonule

For cryo-EM analysis, ciliary zonules were extracted from dissected bovine ciliary zonule tissue and were disrupted using sonication in 20mM Tris-HCl, 400mM NaCl and 2mM CaCl₂ (pH7.4) with two 10-s pulses and cooled on ice for 30s between pulses. Samples were centrifuged and the supernatant was separated using size exclusion chromatography with a 5ml CL-2B resin column. The column was equilibrated in either the sonication buffer or a physiological salt buffer for cryogenic transmission electron microscopy studies (20mM Tris-HCl, 150mM NaCl and 2mM CaCl₂ (pH7.4)). The void volume containing fibrillin microfibrils was saved for further electron microscopy analysis. Each purification utilized the ciliary zonules from a single bovine eye. Separate purifications were performed for the STEM mass mapping and cryo-EM experiments and multiple purifications were used for optimization of cryo-EM grid preparation and data collection.

Fibrillin microfibril extraction from ΔH1 and WMS mice

Wild-type C57BL/6 mice or mice homozygous for either deletion of the first hybrid domain (ΔH1)³⁵ or a deletion of three domains (TB1–PRR–EGF4) that causes WMS³⁶ were maintained at a temperature of 20–24°C under 50–70% relative humidity with a light cycle of 12h day and 12h night. A 1cm² region was dissected from the back skin of 6-week-old males and digested overnight at 4°C in digestion buffer (0.1mgml⁻¹ Collagenase Type I-a (Sigma–Aldrich) in 20mM Tris-HCl, 400mM NaCl and 2mM CaCl₂ (pH7.4)). Samples were centrifuged and separated using size exclusion chromatography as described above. The purification and imaging were repeated at least twice on different skin samples.

Negative stain electron microscopy

Microfibrils extracted from the skin of mice with the mutations and control C57BL/6 mice were adsorbed onto glow-discharged carbon-coated copper grids (Agar Scientific) and stained with 2% uranyl acetate. Grids were imaged at a magnification of 23,000× on a Tecnai G2 Polara TEM (FEI) equipped with a K2 Summit direct detector (Gatan) operating at an accelerating voltage of 300kV. Images were collected over a 1s exposure time in linear mode and sampled at 1.4Åpixel⁻¹. The microfibril repeat was manually picked in RELION-2.1 (ref. ⁵⁷) and subjected to 2D class averaging.

To determine the period length of the H1 and WMS mutated microfibrils, the periodicities of 100 microfibril repeats were measured using ImageJ⁵⁸. Microfibrils were extracted from images and straightened using the straighten tool before measuring the repeat length.

Cryo-EM sample preparation and data collection

Microfibril samples were adsorbed onto glow-discharged holey carbon Quantifoil R1.2/1.3 grids before being blotted and plunge frozen in liquid ethane using a Vitrobot Mark IV (FEI). Microfibrils were imaged using automated data collection in EPU on a Titan Krios electron microscope (FEI) operating at an accelerating voltage of 300kV. A total of 1,310 videos comprising 20 frames with a 20-s exposure time and a total dose of 66eÅ⁻² were collected on a K2 Summit direct detector (Gatan) in counting mode at a nominal magnification of 64,000, which gave a pixel size of 2.2Å. Initial imaging of microfibrils showed that they had a preferred orientation on the grid, so during data collection the stage was tilted to 45°.

Symmetry analysis of 3D maps

Orientation correlation plots were made by rotating the 3D maps refined in RELION-2.1 (pre-postprocessing) about the imposed C2 symmetry axis or the putative symmetry axis for the C1 map (Extended Data Fig. ​Fig.1a).1a). Each map was rotated over a series of angles, from 0 to 360° in increments of 5°, and correlated back to the original unrotated map. Normalized correlation coefficients were calculated in a map region defined by a binary mask derived from the mask used for the refinements. This original mask was symmetrized by rotating sequentially over 5° steps (range 0–360°) to create a series of masks and then taking their sum.

Where two independent half-maps were used, one was kept constant for comparison and the other was rotated around the symmetry axis (Extended Data Fig. ​Fig.1a).1a). The program SPIDER (version UNIX 26.04) was used for the map rotations and correlation coefficient calculations⁵⁹.

Single-particle data processing bead region reconstruction

Videos were motion corrected and dose weighted using MotionCor2 (ref. ⁶⁰). Corrected images were imported into Warp⁶¹ where 27,737 particles were picked using a Warp box net that had previously been trained on manually picked particles of the fibrillin microfibrils. Patch-based contrast transfer function (CTF) estimation was used to calculate local CTF values for the particles. Particle stacks were imported into cryoSPARC⁶² and used in a homogenous refinement using a negative stain reconstruction of the microfibril repeat as an initial model³⁷. The resulting structure from cryoSPARC was then further refined in RELION-2.1 (ref. ⁵⁷). Particles that had been aligned to the full fibrillin repeat were recentered so that the bead or arm region coordinates were then at the particle center using a custom Python script. For the bead region reconstruction, the shifted particle coordinates were then extracted and were 2D classified without alignment to remove the bad particles; 13,184 particles from good classes were selected for 3D classification. The 3D classification of the shifted particles was performed with a restricted angular search using the command --sigma_ang 5. The resulting best class was then further refined using 3D auto-refine with C2 symmetry imposed down the fiber axis. To remove any remaining bad particles, a nonaligned 2D classification was performed and 7,139 particles were used in a final refinement. After postprocessing in RELION, the final structure had a resolution of 9.7Å (Extended Data Fig. ​Fig.1b).1b). Local resolution estimation using the two half-maps from the final bead refinement was performed in cryoSPARC (Extended Data Fig. ​Fig.1d1d).

For the arm region reconstruction, the shifted particle coordinates were also extracted and 2D classified without alignment to remove bad particles; 4,957 good particles were selected for 3D classification. The 3D classification of the shifted particles was then performed with a restricted angular search using the command --sigma_ang 5. The resulting best class was refined using 3D auto-refine with C2 symmetry imposed down the fiber axis, as with the bead reconstruction. After postprocessing in RELION, the final arm structure had a resolution of 18.3Å (Extended Data Fig. ​Fig.4).4). The electron microscopy data have been deposited to the Electron Microscopy Data Bank (EMDB) with accession codes EMD-13984 for the bead model and EMD-13986 for the arm region.

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Extended Data Fig. 4

Fibrillin arm region cryoEM data.

a) A Graph of the Fourier shell correlation (FSC) of the fibrillin microfibril arm structure. Resolution was calculated from the correlation between two independently refined halves of the data and is 18.3Å resolution at 0.143 criterion. b) A 3D representation of the angular distribution of particles used in the arm structure reconstruction.

Refining antibody epitopes with recombinant fibrillin fragments

Recombinant human fibrillin-1 fragments were expressed and purified as previously described^19,63. Proteins were detected by western blotting with the antibodies mab2502 (clone 26) and mab1919 (clone 11C1.3) from Sigma–Aldrich, using a dilution of 1:1,000.

LTBP-1 binding and STEM mass mapping

Full-length human LTBP-1 was purified as previously described⁵⁶ and incubated with bovine fibrillin microfibrils at a 2:1 molar ratio for 4h at 4°C. The complex was adhered for 60s to 400-mesh carbon-coated grids then washed with Milli-Q water three times and dried. The sample was visualized in STEM mode with a Fischione high-angle annular dark-field detector on an FEI Tecnai 12 Twin TEM at 34,000× magnification. A camera length of 350cm was used to give an angular collection range of 20–100mrad. Tobacco mosaic virus was used as a calibration standard for mass per unit length. The electron dose was kept sufficiently low (<300enm⁻¹) to produce negligible mass loss. Mass per unit length measurements and axial mass distributions were measured from STEM annular dark-field images using the Semper6 image analysis software (Synoptics).

Fibrillin–LTBP-1 binding by surface plasmon resonance

The C-terminal region of human LTBP-1 was purified as previously described⁵⁶ and immobilized by amine coupling onto a CM5 sensor chip at 2.5μgml⁻¹ in 50mM sodium acetate buffer (pH3.0) in a Biacore T200 biosensor; typically, 200 response units were immobilized. Recombinant human fibrillin-1 fragments PF3 and PF3 WMS (0–50nM) were injected onto the sensor chip at a flow rate of 50μlmin⁻¹ in 10mM HEPES, 150mM NaCl, 1mM CalCl₂ and 0.05% Tween-20 for 100s and then allowed to dissociate for 180s. Regeneration was performed by injection of 10mM glycine (pH2) for 30s at a flow rate of 30μlmin⁻¹ followed by a stabilization period of 60s. K_d values were calculated using equilibrium analysis: equilibrium response was plotted against concentration and nonlinear regression was used to calculate K_d values using the equation for one-site binding. Each assay was performed at least twice.

Complexing integrin α_vβ₃ with fibrillin microfibrils

Integrin-αv Headpiece M400GC and pcDNA3.1-β3 were gifts from T. Springer (plasmids 159637 and 27289; Addgene)^64,65. The human integrin α_v headpiece (residues 1–594) and the β₃ headpiece (residues 1–472) with a mutation causing the amino acid alteration p.Gln267Cys were subcloned and ligated into the pBudCE4.1 mammalian expression vector. The α_v headpiece contains a C-terminal acid coiled coil and a Twin-Strep tag, whereas the human β₃ headpiece has a C-terminal base coiled coil and a His tag.

The recombinant construct was transiently transfected into the Expi293 mammalian expression system (Thermo Fisher Scientific) according to the user guide. The integrin α_vβ₃ headpiece was then affinity purified using Strep-Tactin XT 4Flow resin (IBA Lifesciences), followed by size exclusion chromatography on a Superdex 200 increase column (Cytiva) equilibrated in buffer containing 20mM HEPES and 150mM NaCl (pH7.5).

Bovine ciliary zonule microfibrils and integrin α_vβ₃ were incubated together in an approximate 2:1 integrin-to-microfibril molar ratio in 20mM Tris-HCl, 150mM NaCl, 500μM Mn²⁺ and 500μM Ca²⁺ (pH7.4) for 1h at 4°C. Microfibrils with and without integrin α_vβ₃ were then imaged using negative stain electron microscopy as described above.

We thank staff at the Electron Microscopy Core Facility (RRID:SCR_021147; Faculty of Biology, Medicine and Health, University of Manchester) for assistance and the Biotechnology and Biological Sciences Research Council (BB/T017643/1) for funding toward the Glacios cryo-EM used for screening. The Wellcome Trust Centre for Cell-Matrix Research is supported by funding from the Wellcome Trust (203128/Z/16/Z). A.R.F.G. was supported by Biotechnology and Biological Sciences Research Council funding (BB/N015398/1 to C.B., A.M.R. and M.J.S. and BB/S015779/1 to C.B.). We acknowledge the UK national Electron Bio-Imaging Centre (eBIC) for access to cryo-EM facilities (EM16619-5). Data were collected at the Astbury Biostructure Laboratory on FEI Titan Krios microscopes, which were funded by the University of Leeds and Wellcome Trust (108466/Z/15/Z). Funding for this study was also provided by Deutsche Forschungsgemeinschaft project numbers 73111208 (SFB 829/B12), 384170921 FOR2722/C2 and 397484323 TRR259/B09 to G.S.