Introduction

Understanding how cells regulate the size of their organelles is a fundamental question in cell biology. However, the three-dimensional complexity of most organelles poses challenges for accurate measurement, and thus, the underlying regulation mechanisms remain largely elusive. In contrast to the localization of most organelles within cells, cilia (also known as flagellar) are microtubule-based structures that extend from the cell surface, facilitating a more straightforward quantification of their size. Cilia are highly conserved organelles found across various organisms, ranging from protozoa to humans. Their formation relies on microtubules, and their size can be easily measured by their length, making cilia an ideal model for studying size regulation of sub-cellular organelles within the same organisms (Chan and Marshall, 2012).

Cilia play a crucial role in regulating various physiological and biochemical processes (Goetz and Anderson, 2010; Nachury and Mick, 2019; Singla and Reiter, 2006). Structural or functional abnormalities of this organelle can result a wide range of human genetic disorders, including retinal degeneration, polycystic kidneys, and mental retardation (Mill et al., 2023; Reiter and Leroux, 2017; Song et al., 2016). The assembly and maintenance of cilia rely on an elaborate process known as intraflagellar transport (IFT) (Kozminski et al., 1993). The IFT complex is located between the doublet microtubules of the cilia and the ciliary membrane, playing a vital role as a mediator of cargo transportation within cilia (Bhogaraju et al., 2013; Hesketh et al., 2022; Meleppattu et al., 2022). The IFT complex consists of two subcomplexes: the IFT-B complex, which transports the precursors required for cilia assembly from the base to the tip, powered by Kinesin-2; and the IFT-A complex, which transports axonemal turnover products back to the cell body by binding to dynein (Kardon and Vale, 2009; Ou et al., 2007; Scholey and J., 2008; Taschner et al., 2012). Electron microscopy studies have suggested that multiple IFT particles move together along the axoneme, earning the name “IFT trains” (Jordan et al., 2018; Kozminski et al., 1995; Stepanek and Pigino, 2016). In Caenorhabditis elegans, both the slow-speed heterotrimeric kinesin II and the fast-speed homodimeric kinesin OSM-3 coordinate IFT, ensuring the assembly of sensory cilia (Snow et al., 2004). The IFT system also interacts with the BBSome complex, dysfunction of which is associated with the human ciliopathy Bardet-Biedl syndrome. The BBSome complex is moved by IFT and functions to maintain the physical connection between IFT-A and IFT-B subcomplexes in C. elegans (Ou et al., 2005). Moreover, the BBSome is involved in diverse functions, including protein trafficking into and out of the cilia. (Berbari et al., 2008; Jin et al., 2010; Lechtreck et al., 2009; Liu et al., 2021; Nachury et al., 2007; Ye et al., 2018).

The intraflagellar transport system plays a crucial role in ciliogenesis and is highly conserved across various organisms. Interestingly, the length of cilia exhibits significant diversity in different models. For example, Chlamydomonas has two flagella with lengths ranging from 10 to 14 μm, while sensory cilia in C. elegans vary from approximately 1.5 μm to 7.5 μm. In most mammalian cells, the primary cilium typically measures between 3 and 10 μm. Considering the conserved structure of cilia, it becomes intriguing to understand how their length is regulated in different cell types. Extensive research into flagellar length regulation has been conducted in Chlamydomonas. After one or two flagella are abscised, the shorter flagella can regenerate to their original length. During this regeneration process, the short flagella undergo a rapid growth phase, transitioning to a slower elongation phase as they approach their steady-state length (Rosenbaum et al., 1969). IFT plays a central role in mediating flagellar regeneration and IFT particles usually assemble into ’long’ and ’short’ trains within the flagella. At the onset of flagellar growth, long trains are prevalent, while the number of short trains gradually increases as the flagellum elongates (Engel et al., 2009; Vannuccini et al., 2016). Moreover, the rate at which IFT trains enter the flagella, known as the IFT injection rate, is negatively correlated with flagellar length during regeneration (Engel et al., 2009; Ludington et al., 2013). Researchers have proposed and tested several theoretical models to explain the regulatory mechanism of the IFT injection rate (Ishikawa et al., 2023; Marshall, 2023; Wemmer et al., 2020). Intriguingly, recent studies in the parasitic protist Giardia, which possesses eight flagella of varying lengths, revealed that the ciliary tip localization of microtubule-depolymerizing kinesin-13 is inversely correlated with flagellar length, similar to its role in flagellar length regulation (McInally et al., 2019; Piao et al., 2009; Wang et al., 2013). These findings add another layer of complexity to our understanding of ciliary length regulation and underscore the importance of investigating diverse model organisms to gain comprehensive insights into this fundamental biological process.

Notably, most studies on ciliary length control have focused on single-celled organisms. However, in vertebrates, the presence of highly diverse cell types results in cilia of varying lengths. Understanding how cilia length is regulated in different cell types and why such diversity exists is essential for comprehending the pathogenic mechanisms underlying various organ defects seen in ciliopathies. Unfortunately, direct observation of intraflagellar transport (IFT) in living vertebrates has posed challenges, limiting our knowledge in this area.

In this study, we capitalized on the benefits of embryonic transparency in zebrafish to explore dynamic IFT in various types of cilia. To the best of our knowledge, this is the first report of IFT investigation in multiple organs within a living organism. Our findings revealed a positive correlation between the speed of IFT transport and cilia length. Furthermore, ultra-high-resolution microscopy showed a close association between cilia length in different organs and the size of IFT fluorescent particles, indicating the presence of larger IFT trains in longer cilia. This observation suggests that cargo and motor proteins are more effectively coordinated in transporting materials, resulting in increased IFT velocity—a novel regulatory mechanism governing IFT speed in vertebrate cilia.

Results and Discussion

Zebrafish provide an ideal model to compare ciliogenesis in different organs

Similar to humans, cilia are widely present in various organs in zebrafish. Utilizing an Arl13b-GFP transgene under the control of the beta-actin promoter, we can observe cilia in live embryos within organs such as Kupffer’s vesicle, ear, lateral line, spinal cord, and skin. Cilia in the pronephric duct, olfactory pit, photoreceptor cells, and sperms can be visualized through antibody staining with acetylated-tubulin. Notably, the number and length of cilia exhibit significant variation across different tissues (Fig 1). While most cells contain a single cilium, certain specialized cell types, including olfactory epithelia and pronephric duct, form multiple cilia. In adult zebrafish, multiciliated cells can also be found in the brain ventricles (ependymal cells) and ovary(Ogino et al., 2016). Consequently, zebrafish provides an ideal model for investigating ciliogenesis in diverse cell types (Song et al., 2016).

Diverse type of cilia are present in zebrafish

(A) Cilia in the kupffer’s vesicle (KV) of a 10-somite stage zebrafish larvae. (B-H) Confocal images showing cilia in different type of cells as indicated. The position of these cells were indicated in the top diagram. (I-J) Confocal images showing cilia in the sperm (flagellum) or spermatocyte. All the cilia were visualized with anti-acetyleated tubulin antibody. Scale bar=10 μm.

Rescue of ovl (ift88) mutants with Tg(hsp70l:ift88-GFP) transgene

To visualize IFT in zebrafish, we first generated a stable transgenic line, Tg(hsp70l:ift88-GFP), which expresses a fusion protein of Ift88 and GFP under the control of the heat shock promoter (Fig. 2A). Ift88 plays a crucial role as a component of the IFT complex in maintaining ciliogenesis. Zebrafish ovl mutants exhibited body curvature defects and typically do not survive beyond 7 days post-fertilization (dpf) (Tsujikawa and Malicki, 2004). By performing a daily heat shock starting from 48 hours post-fertilization (hpf), we observed that the body curvature defects were completely rescued at 5dpf (Fig 2B, C). Furthermore, we assessed ciliogenesis defects in these mutants. At 5 dpf, cilia were absent in most tissues of the ovl mutants (Fig. 2D). In contrast, this transgene effectively rescued ciliogenesis defects in all examined tissues (Fig. 2D and S1A). Interestingly, the GFP fluorescence of the transgene was prominently enriched in the cilia (Fig 1D). Additionally, we conducted continuous heat shock experiments, which showed that ovl mutants carrying this transgene were able to survive to adulthood (Fig. S1B). Taken together, these findings demonstrate that Ift88-GFP can substitute for endogenous Ift88 in promoting ciliogenesis.

Rescue of ovl mutants with Tg(hsp70l:ift88-GFP) transgene.

(A) Schematic diagram of hsp70l:ift88-GFP construct. (B) Procedure of heat shock experiments for ovl mutants rescue assay. (C) External pheontype of 3dpf wild type, ovl mutant or ovl mutant larvae carrying Tg(hsp70l:ift88-GFP) transgene. The numbers of larvae investigated were shown on the bottom right. (D) Confocal images showing cilia in different type of organs as indicated. Red channel indicates cilia visualized by anti-acetylated α-tubulin antibody and fluorescence of Tg(hsp70l:ift88-GFP) is showed in green. Scale bars: 200 μm in panel C and 10 μm in panel D.

Visualization of IFT in different cilia

The enrichment of Ift88-GFP within cilia implies that the Tg(hsp70l: ift88-GFP) transgene could serve as a valuable tool for real-time observation of IFT movement (Fig 2D). Despite cilia typically being situated in the deep regions of the body, we managed to detect the movement of GFP fluorescence particles using a high-sensitive spinning-disc microscope. First, we focused on ear cristae hair cell cilia which are longer and easy to detect. We succeeded in the direct visualization of the movement of fluorescent particles in these cilia (Movie S1). Kymograph analysis revealed bidirectional movement of the Ift88-GFP particles along the cilia axoneme (Fig 3A), akin to IFT movements observed in other species (Kozminski et al., 1993; Orozco et al., 1999). Moreover, we also captured the dynamic movement of these Ift88-GFP particles in various cilia, including those of neuromasts, pronephric duct, spinal cord, and skin epidermal cells (Fig 3B-E, Movies S2-5). These movies provide a great opportunity to compare IFT across different cilia.

Intraflagellar transport in different type of cilia.

(A-E) Left, Snapshot of Intraflagellar transport videos in different cell types as indicated. Middle (A, B), Snapshot of same cilia at different time points. Arrowheads with the same color indicate the same IFT particle. Right, kymographs illustrating the movement of IFT particles along the axoneme. Horizontal scale bar: 10 μm and vertical scale bars: 10 s. Representative particle traces are marked with white lines in panels D and E. (F) Histograms displaying the velocity of anterograde and retrograde IFT in different type of cilia as indicated. “Antero.” and “Retro.” represent anterograde and retrograde transport, respectively. (G) Summary of IFT velocities in different tissues of zebrafish. Numbers of IFT particles are shown in the brackets. (H) Left, Statistics analysis of cilia length in different tissues of zebrafish. Right, anterograde and retrograde IFT average velocity in different tissues of zebrafish. (I)Anterograde and retrograde IFT velocities plotted versus cilia length. Linear fit (black line) and coefficient of determination are indicated. (J) Frequency of anterograde and retrograde IFT entering or exiting cilia.

Correlation between IFT speed and ciliary length

To characterize the dynamics of IFT, we quantified their movement speed using kymographs generated from recorded movies (Fig. 3F, G). Within each type of cilia, the retrograde IFT showed higher speed compared to anterograde transport, consistent with previous findings in C. reinhardtii and C. elegans, where dynein motors were found to move faster than Kinesin motors. Surprisingly, we observed significant variability in IFT velocities among different cilia. In ear crista cilia, the average speed of anterograde IFT was 0.68 μm/s, while in the cilia of neuromast hair cells, it decreased to 0.54 μm/s. In skin epidermal cilia and spinal canal cilia, the transport rates were further reduced to 0.42 μm/s and 0.33 μm/s, respectively. The pronephric duct cilia showed intermediate average anterograde IFT rates at 0.46 μm/s. Similarly, retrograde transport also displayed considerable variability, with ear crista and neuromast cilia exhibiting the highest speeds (1.55 μm/s and 1.47 μm/s, respectively). In contrast, cilia in the spinal canal showed the slowest IFT, with an average speed of 0.35 μm/s, which was less than one fourth of the speed observed in ear crista cilia (Fig 3G).

Both anterograde and retrograde IFT displayed remarkably high transport speeds in ear crista and neuromast cilia. Intriguingly, we observed that these cilia were particularly longer compared to others. To investigate this correlation further, we compared ciliary length in different tissues and discovered a strong correlation between cilia length and IFT speeds (Fig 3H, I). Specifically, longer cilia demonstrated faster IFT rates in both the anterograde and retrograde directions. Interestingly, longer cilia also have a higher frequency of fluorescent particles entering cilia (Fig 3J). These findings establish a compelling link between ciliary length and IFT speeds, suggesting a potential functional significance. To validate this relationship further, we created an additional transgenic line, Tg(βactin2: tdTomato-ift43), which allowed us to label Ift43, a constituent of the IFT-A complex. Through the analysis of Ift43 transport in this transgenic line, we reaffirmed that the tdTomato-Ift43 fluorescence particles also exhibited the highest transport speeds in ear crista cilia (Fig S2).

IFT in the absence of Kif17 or Bbs proteins

To understand the potential mechanisms underlying the variation in IFT speeds among different cilia, we initially focused on differences in motor proteins. In C. elegans, the homodimeric kinesin-2, OSM-3, drives the IFT complex at a relatively higher speed compared to the heterotrimeric Kinesin-2 (Ou et al., 2005). We examined IFT in kif17 mutants, which carry a mutation of the fast homodimeric kinesin (Zhao et al., 2012). Surprisingly, in the absence of Kif17, the IFT speeds remained similar to those of control larvae (Fig 4A, B, S3, Movie S6, Table S1). Similarly, the IFT maintained regular speed in the absence of Kif3b in the ear crista(Fig 4A, B, Movie S7, Table S1), possibly due to the redundant function of Kif3c in the heterotrimeric Kinesin-2 (Zhao et al., 2012). Additionally, we assessed IFT in the bbs4 mutants, which has been proposed to affect the connection between the two IFT subunits in C. elegans. Once again, the Bbs4 mutation had little effect on IFT motility (Fig 4A, B, S3, Movie S8, Table S1). Thus, these data suggest that the variability in IFT speeds among different cilia cannot be attributed to the use of different motor proteins or the involvement of the BBSome complex.

Alterations in motor proteins, BBS proteins, or tubulin modifications have minimal effects on IFT.

(A) Left: Snapshot of IFT videos in crista cilia of 4dpf wild type or mutant larvae as indicated. Right: Kymographs showing IFT particle movement along axoneme visualized with Ift88:GFP. Horizontal scale bar: 10μm and vertical scale bar:10s. (B) Histograms showing anterograde and retrograde IFT velocity in crista cilia of control or mutant larvae. (C) Genomic structure and sequences of wild type and ttll3 mutant allele. PAM sequence of sgRNA target are indicated in blue. (D) Protein domain of Ttll3 in wildtype and ttll3 mutants. (E) Confocal images showing crista cilia in wild-type or maternal-zygotic (MZ) ttll3 mutants visualized with anti-monoglycylated tubulin antibody (green) and anti-acetylated α-tubulin antibody (red). (F) Histograms depicting IFT velocity in crista cilia of control and ttll3 mutants. Top, anterograde IFT. Bottom, retrograde IFT. (G) Histograms illustrating IFT velocity in crista cilia of ccp5 or ttll6 morphants. Scale bars: 10 μm in panel A and 5 μm in panel E. *p<0.5; *** p<0.001.

Tubulin modifications, ATP concentration and IFT

IFT was driven by kinesin or dynein motor proteins along the ciliary axoneme. The post-translational modifications of axonemal tubulins can affect the interaction between microtubules and motor proteins, thereby regulating their dynamics (Hong et al., 2018; Janke and Bulinski, 2011; O’Hagan et al., 2017; Sirajuddin et al., 2014). Next, we asked whether tubulin modifications can affect IFT in zebrafish. Ttll3 is a tubulin glycylase that are involved in the glycylation modification of ciliary tubulin (Wloga et al., 2009). We generated zebrafish ttll3 mutants and identified a mutant allele with an 8bp insertion, which causes frameshift, resulting in a significantly truncated Ttll3 protein without TTL domain (Fig. 4C,D). Immunostaining with anti-monoglycylated or polyglycylated tubulin antibody revealed that the glycylation modification was completely eliminated in all the cilia investigated (Fig. 4E and S4). Surprisingly, there are no obviously defects in the number and length of cilia in the mutants. The velocity of IFT within different cilia was also seems unchanged (Fig. 4F, Movie S9, Table S1). Moreover, the mutants were able to survive to adulthood and there is no difference in the fertility or sperm motility between mutants and control siblings, which is slightly different to those observed in mouse mutants (Gadadhar et al., 2021).

Next, we investigated whether polyglutamylation of axonemal tubulins can regulate IFT movement in zebrafish. First, we knocked down the expression of ttll6, which has been shown early to reduce tubulin glutamylation and resulted in body curvature in zebrafish (Fig. S5A, B) (Pathak et al., 2011). The efficiency of ttll6 morpholinos was confirmed via RT-PCR (reverse transcription-PCR), which showed the splicing error of intron 12 when introduced the morpholinos (Fig. S5C, D). Interestingly, we observed only minor differences in IFT velocity between ttll6 morphants and control groups (Fig 4G, Table S1). Similarly, the IFT speeds also exhibited only slightly changes in ccp5 morphants, which decreased the deglutamylase activities of Ccp5 and resulted in a hyper-glutamylated tubulin (Fig. 4G and S5E-H, Table S1) (Pathak et al., 2014). Together, these results suggest that tubulin codes may play relatively minor roles on IFT in zebrafish. Considering the big difference in the IFT speed among different cilia, we think it is very unlikely such difference is caused by different levels of tubulin modification.

The movement of kinesin and dynein motors relies on the energy derived from ATP hydrolysis. In vitro studies using molecular force clamp techniques have shown that increasing ATP concentration significantly enhances the speed of kinesin during cargo loading (Visscher et al., 1999). We further examined whether the difference of IFT speeds was caused by variation of ATP concentration inside cilia. We generated an ATP reporter line, Tg (βactin2: arl13b-mRuby-iATPSnFR1.0), which contains a ciliary localized ATP sensor, mRuby-iATPSnFR1.0 driven by b-actin2 promotor (Fig. S6A-B) (Lobas et al., 2019). This ATP sensor utilizes relative fluorescence intensity to indicate the concentration of ATP. By measuring the ratio of mRuby red fluorescence to green fluorescence in the longer crista and shorter epidermal cilia, we compared relative ATP levels between these two types of cilia. Again, we found no difference in the ATP concentration between crista and epidermal cilia, suggesting that variation of ATP concentration was unlikely to be the cause of different IFT speed (Fig. S6C).

Larger IFT particles in longer cilia

Finally, we aim to investigate the size of IFT particles within different type of cilia. In the flagellar of Chlamydomonas, IFT particles are usually transported as IFT trains, consisting of multiple IFT-A and IFT-B repeating subcomplexes and the kinesin-2 and IFT dynein motors. However, with current technique, it is unfeasible to distinguish the size of IFT trains on different type of cilia through ultra-structure electron microscopy in zebrafish. Instead, we sought to compare the size of the fluorescence particles using STED ultra-high-resolution microscopy. With this method, we were able to identify single IFT fluorescence particles with relatively high resolution. Compared with regular spinning disk data, the number of IFT fluorescence particles was significantly increased in the cilia (Fig 5A, B). When comparing the size of these fluorescence particles, we found that the particle sizes were significantly larger in the longer crista cilia than those of the shorter spinal cord cilia (Fig. 5C).

Increased size of IFT fluorescent particles in crista cilia.

(A) Representative STED images of crista (top) and spinal cord (bottom) in 4dpf Tg(hsp70l: ift88-GFP) larva. Cilia was stained with anti-monoglycylated tubulin (magenta), and IFT88-GFP particles were counterstained with anti-GFP antibody (green). Enlarged views of the boxed region are displayed on the right. (B) Dot plots showing the number of IFT particles per arbitrary unit (a.u.) in crista cilia recorded by spinning disk and STED. (C) Statistical analysis showing IFT particles size in the cilia of ear crista and spinal cord. (D) External phenotypes of 2 dpf zebrafish larvae injected with higher and lower dose of ift88 morpholinos. (E) Statistical analysis of cilia length in control or ift88 morphants. (F) STED images showing IFT particles in crista cilia of 3dpf control or ift88 morphants. Enlarged views of the boxed region are displayed on the right. (G) Dot plots showing the number of IFT particles in control and ift88 morphants. (H) Statistical analysis showing IFT particles size of crista cilia in control or ift88 morphants. (I) Left, Snapshot of IFT videos in crista cilia of 3dpf control (top) or ift88 morphant (bottom) carrying Tg(hsp70l: ift88-GFP). Right, Kymographs showing movement of IFT particles along axoneme. Horizontal scale bar: 10μm and vertical scale bar:10s. (J) Histograms showing IFT velocity in 3dpf control or ift88 morphants. (K) Model illustrating IFT with different train sizes in long and short cilia. Scale bars: 0.2 μm in panel A and F, and 500 μm in panel I. **p<0.01; *** p<0.001.

To further test whether the higher IFT velocity was associated with large IFT particles in the crista cilia, we performed morpholino based knockdown analysis. Injection of ift88 morpholino caused body curvature due to ciliogenesis defects (Fig 5D). When injecting lower dose of ift88 morpholino, we found zebrafish embryos can still maintain grossly normal body axis, while cilia in ear crista became significantly shorter (Fig 5D, E, I). Due to partial loss of Ift88 proteins, the number of IFT complex decreased significantly as suggested by the reduced number of IFT fluorescence particles in the morphant cilia (Fig 5F, G). Noticeably, the size of the fluorescent particles also decreased significantly, implying a potentially reduced length of the IFT trains (Fig. 5F, H). Strikingly, we found the IFT speed also decreased significantly in the shorter cilia (1.55 μm/s in control vs 1.18 μm/s in morphants) (Fig 5I, J, Movie S10). Taken together, these data strongly suggested that the size of IFT fluorescence particles is closely related to IFT speed and longer cilia are prone to contain larger IFT particles than shorter cilia.

A hypothetical model of cilia length regulation in zebrafish

With its diverse array of cilia types, zebrafish provide an exceptional model for investigating the intricate mechanisms underlying ciliary length regulation. By creating a transgenic line that expresses ciliary-targeted IFT proteins, we have demonstrated a positive correlation between IFT transport speed and the length of cilia. To the best of our knowledge, this study represents the first instance of comparing IFT transport in cilia from different types of organs within the same organism. Interestingly, certain conventional factors known to govern IFT transport regulation in C. elegans or Chlamydomonas appear to exert limited influence in zebrafish. Firstly, IFT transport speed showed no discernible connection to ciliary motility, as evidenced by the comparable IFT speeds observed in both motile spinal cord cilia and primary cilia of the skin’s epidermal cells (Fig 3). Furthermore, the accelerated IFT transport cannot be attributed to distinct motor utilization, BBS proteins, or tubulin modifications, all of which have been suggested to regulate IFT transport in worms. Surprisingly, tubulin glycylation is not only non-essential for IFT transport but also dispensable for zebrafish development, as zebrafish ttll3 mutants are viable and fertile. Collectively, these results suggest that the regulation of IFT velocity in zebrafish cilia differs from that observed in C. elegans, thereby highlighting the intricate complexity of IFT regulation across various organisms.

Remarkably, our studies revealed that the IFT fluorescence particles were significantly larger in longer crista cilia than those of shorter cilia. The IFT complex typically travels as trains, with multiple repeating IFT units being transported simultaneously. The increased size of the fluorescence particles implies that longer cilia might form larger IFT trains for more effective cargo transportation. Decreasing the quantity of IFT88 proteins could diminish the likelihood of IFT complex assembly, consequently leading to a reduction in the size of IFT trains. Importantly, the size of IFT particles was significantly reduced in ift88 morphants, concurrent with the decreased transport speed of IFT. Thus, our data support a length control model for cilia that operates through the modulation of IFT train size (Fig 5K). Within longer cilia, the IFT complex appears predisposed to form lengthier repeating units, thereby creating an optimal platform for efficient transport. This environment enhances the coordination between cargos and motor proteins, resulting in an improved transportation speed. This orchestration potentially involves the synchronization of motor proteins, ensuring their precise functionality and directional alignment during transport—a concept supported by various models (Stukalin et al., 2005; Urnavicius et al., 2018). Furthermore, insights from the cryo-EM structure of intraflagellar transport trains have suggested that each dynein motor protein might propel multiple IFT complexes. For instance, the ratio of dynein: IFT-B: IFT-A in the flagella of Chlamydomonas is approximately 2:8:4 (Jordan et al., 2018). It remains plausible that longer cilia in vertebrates could recruit a higher ratio of motor proteins to execute IFT, thus intensifying the driving force for cargo transport. The mechanisms behind achieving these conditions may require further investigation.

Materials and methods

Ethics statement

All zebrafish study was conducted according standard animal guidelines and approved by the Animal Care Committee of Ocean University of China (Animal protocol number: OUC2012316).

Zebrafish Strains

All zebrafish strains were maintained following standard protocols. The following mutant strains were used: ovl (Tsujikawa and Malicki, 2004), kif3b and kif17 (Zhao et al., 2012). Three transgenic lines, Tg(hsp70l:ift88-GFP), Tg(βactin2:tdTomato-ift43) and Tg (βactin2: arl13b-mRuby-iATPSnFR1.0), were generated in this study. The constructs for making these transgene were created using Tol2 kit Gateway-based cloning (Kwan et al., 2007). The ttll3 mutants were generated via CRISPR/Cas9 technology with the following target sequence: 5’-GGGTGGAGCGGCGATTGCCA-3’. The bbs4 mutants were generated by TALEN system with the following binding sequences: 5’-TAAACTTGGCATTACAGC-3’ and 5’-TCCCAGCATCATGTAGGTC -3’. All strains involved are stable lines.

IFT imaging and analysis

For crista cilia imaging, zebrafish larvae were anesthetized with 0.01% Tricaine in E3 water and then embedded in 1.25% low melting point agarose on a confocal dish. When imaging cilia in neuromast, epidermal cells, spinal cord, or pronephric duct epithelial cells, the embryos were anesthetized and placed on a confocal dish. Excess water was carefully removed, and a circular cover glass was then placed over the sample for imaging. IFT movements in crista cilia and neuromast were recorded using an Olympus IX83 microscope equipped with a 60X, 1.3 NA objective lens, an EMCCD camera (iXon+ DU-897D-C00-#BV-500; Andor Technology), and a spinning disk confocal scan head (CSU-X1 Spinning Disk Unit; Yokogawa Electric Corporation). Time-lapse images were continuously collected with 100 or 200 repeats using μManager (https://www.micro-manager.org) at an exposure time of 200 ms. Kymographs were generated using Image J software. IFT Movement in cilia of epidermal cells, spinal cord, and pronephric duct epithelial cells were recorded using an Olympus IX83 microscope equipped with a 100X, 1.49 NA objective lens, and the same EMCCD camera and spinning disk confocal modules as mentioned above.

Whole-mount Immunofluorescence

Zebrafish larvae were fixed overnight at 4°C in 4% PFA. After removing the fixative, they were washed three times with PBS containing 0.5% Tween 20 (PBST) and then incubated in acetone for 10 minutes for permeabilization. Subsequently, the embryos were treated with a blocking reagent (PBD with 10% goat serum) for 1 hour and sequentially labeled with primary and secondary antibodies (at a 1:500 dilution) overnight at 4 °C. The following antibodies were used: anti-acetylated α-tubulin (Sigma T6793), anti-monoglycylated tubulin antibody, clone TAP 952 (Sigma MABS277), anti-polyglycylated tubulin antibody, clone AXO49 (Sigma MABS276), anti-GFP (Invitrogen A-11120), and anti-HA (Invitrogen).

Morpholino knockdown

The following morpholinos were used: ttll6 (5’ - GCAACTGAATGACTTACTGAGTTTG - 3’), ccp5 (5’ -TCCTCTTAATGTGCAGATACCCGTT-3’) and a standard control morpholino (5’ - CCTCTTACCTCAGTTACAATTTATA-3’). All morpholinos were purchased from Gene Tools (Philomath, OR). To detect splicing defects caused by morpholinos, we extracted total RNA from 24hpf embryos and performed RT-PCR using the following primer sequences: ttll6 Forward: 5’-AAAGTATTTCCAACACAGCAGCTC-3’, Reverse: 5’-GTGGTCGTGTCTGCAGTGTGGAGG-3’; ccp5 Forward: 5’-TCCTGTCGTTTGTTCATCGTCTGC-3’, Reverse: 5’-CTTAAAGACGAACATGCGGCGAAG-3’

Super-resolution microscopy

High resolution images were acquired using Abberior STEDYCON (Abberior Instruments GmbH, Göttingen, Germany) fluorescence microscope built on a motorized inverted microscope IX83 (Olympus UPlanXAPO 100x, NA1.45, Tokyo, Japan). The microscope is equipped with pulsed STED lasers at 775 nm, and with 561 nm and 640 nm excitation pulsed lasers. Zebrafish larvae were collected and fixed in 4% PFA overnight at 4°C. For STED imaging, the following secondary antibody were used: goat anti-mouse Abberior STAR RED and goat anti-rabbit Abberior STAR ORANGE. The embryos were incubated in secondary antibody(1:100) in blocking buffer at room temperature for 2 h. After wash three times (5 min each) with PBST, larvae were cryoprotected in 30% sucrose overnight. Sagittal sections were collected continuously at 40 μm thickness on Leica CM1850 cryostat. Place the slices at 37 degrees for 1 hour to dry. Rehydrate in PBST for 5 min and cover with Abberior Mount Liquid Antifade. After sealing, the slices were placed at 4 ℃ overnight before imaging.

Statistical analysis

Statistical analysis was performed using GraphPad Prism 8 software. ImageJ software was used to measure length of cilia, fluorescence intensity and particle size. Statistical significance was evaluated by means of the two-tailed Student t-test for unpaired data.

Acknowledgements

We thank Dr. Guangshuo Ou and members of the Zhao lab for their kind help during the preparation of this manuscript. We are also grateful for the excellent support from the core facilities of IEMB at OUC. This work was supported by the National Natural Science Foundation of China (Nos. 32125015, 31991194 to C.Z. and No. 32100661) to H.X.) to C.Z..

Supplementary figures

Rescue of ciliogenesis defects in ovl (ift88) mutants via Tg(hsp70l:ift88-GFP)

(A) Rescue of ciliogenesis defects in ear macula, olfactory placode and pronephric duct. MC, multicilia. Red channel shows cilia visualized by anti-acetylated α-tubulin antibody. Fluorescence of Tg(hsp70l:ift88-GFP) is showed in green. Scale bar=10μm. (B) External phenotypes of adult ovl homozygotes rescued with Tg(hsp70l:ift88-GFP) transgene.

Generation of Tg (βactin2:tdTomato-ift43) transgene for IFT imaging

(A) Schematic diagram showing βactin2:tdTomato-ift43 transgenic construct. (B-C) Left, Snapshot of Intraflagellar transport videos in cilia of ear crista and pronephric duct epithelial cells. Right, kymographs illustrating the movement of IFT particles along the axoneme. Horizontal scale bar=10 μm. Vertical scale bar=10 s. (D) Summary of the anterograde and retrograde velocities of IFT measured in embryos expressing Tg(βactin2:tdTomato-ift43). Numbers of IFT particles are shown in the brackets.

IFT in the cilia of neuromast hair cells of different zebrafish mutants.

(A)(Left) Snapshot of IFT videos in neuromast cilia of 4dpf control, kif17 or bbs4 mutants. (Right) Kymographs showing IFT particle movement along axoneme.(B) Histograms showing anterograde and retrograde IFT velocity in neuromast cilia in control and mutants. Horizontal scale bar=10μm. Vertical scale bar=10s

Complete loss of tubulin glycylation in ttll3 mutants.

(A) Immunostaining with anti-monoglycylated tubulin antibody in 4dpf ttll3 mutants showing complete absence of monoglycylation modification in cilia of neuromast, olfactory placode and pronephric duct. (B) Immunostaining with anti-polyglycylated tubulin antibody revealed complete elimination of polyglycylation modification in multicilia of olfactory placode and pronephric duct. Red channel shows cilia visualized with anti-acetylated α-tubulin antibody. Scale bar=5 μm.

Validation of the efficiency of ttll6 and ccp5 morpholinos.

(A, B, E ,F) External phenotypes of control, ttll6 and ccp5 morphant embryos at 2 dpf. (C) Agarose gel electrophoresis of RT-PCR amplicons using primer pairs as indicated in panel (D). The PCR product size in the ttll6 morphants was significantly larger than that in the control (con.). (D) Schematic diagram of ttll6 sp MO target sites (orange) and RT-PCR primer positions. Sequencing results indicated that ttll6 morphant exhibited incorrect splicing, with intron12 being wrongly included in the mature mRNA.(G) Agarose gel analysis of RT-PCR amplicons using primer pairs as indicated in panel (H). The PCR product size in the ccp5 morphant was significantly larger than that in the control (con.). (H)Schematic diagram illustrating the splice donor sites targeted by antisense morpholinos (orange). Injection of ccp5 MO resulted in the production of aberrant transcripts, wherein intron 5 was mis-spliced into the mature mRNA. Scale bar =500 μm.

Generation of ATP reporter transgenic line.

(A) Schematic diagram of βactin2: arl13b-mRuby-iATPSnFR1.0 transgenic construct. (B) Confocal images showing cilia of crista and epidermal cell in 4dpf transgenic embryos. (C) Statistical results of relative fluorescence intensity in cilia of crista and epicell cells (ratio of red fluorescence intensity vs green fluorescence intensity).

Summary of IFT average velocities in different zebrafish muants or morphants.

Supplementary Videos

Time-lapse images were continuously collected at an exposure time of 200 ms. The display rate was 20 frames per second. Scale bar: 10 μm.

Video 1: Fluorescence time-lapse movie of ear crista cilia visualized by Tg(hsp70l: ift88-GFP).

Video 2: Fluorescence time-lapse movie of neuromast cilia visualized by Tg(hsp70l: ift88-GFP).

Video 3: Fluorescence time-lapse movie of pronephric duct cilia visualized by Tg(hsp70l: ift88-GFP).

Video 4: Fluorescence time-lapse movie of spinal cord cilia visualized by Tg(hsp70l: ift88-GFP).

Video 5: Fluorescence time-lapse movie of skin epidermal cells cilia visualized by Tg(hsp70l: ift88-GFP).

Video 6-9: Fluorescence time-lapse movies of ear crista cilia in kif17, kif3b, bbs4 and ttll3 mutants visualized by Tg(hsp70l: ift88-GFP).

Video 10: Fluorescence time-lapse movies of ear crista cilia in Tg(hsp70l: ift88-GFP) embryos injected with lower dose of ift88 morpholinos.