Disruption of adaptor protein 2μ (
            <scp>AP</scp>
            ‐2μ) in cochlear hair cells impairs vesicle reloading of synaptic release sites and hearing

Jung, Sangyong; Maritzen, Tanja; Wichmann, Carolin; Jing, Zhizi; Neef, Andreas; Revelo, Natalia H.; Al-Moyed, Hanan; Meese, Sandra; Wojcik, Sonja M.; Panou, Iliana; Bulut, Haydar; Schu, Peter; Ficner, Ralf; Reisinger, Ellen; Rizzoli, Silvio O.; Neef, Jakob; Strenzke, Nicola; Haucke, Volker; Moser, Tobias

doi:10.15252/embj.201591885

Cited by 88 publications

(165 citation statements)

References 54 publications

(101 reference statements)

Supporting

Mentioning

149

Contrasting

Unclassified

Order By: Relevance

“…Next, we moved on to early postnatal injections (Fig A, middle and lower, postnatal day 5–7) into the cochlea via the round window, which had proven highly successful for transduction of hair cells (e.g., Akil et al , ; Jung et al , ). We employed AAV‐PHP.B, a novel AAV serotype (Deverman et al , ) with improved efficiency of neural transduction, for expression of Chronos‐ES/TS and Chronos (hSyn promoter, comparable titers, 10 12 GC/ml) in SGNs.…”

Section: Resultscontrasting

confidence: 99%

Ultrafast optogenetic stimulation of the auditory pathway by targeting‐optimized Chronos

et al. 2018

Self Cite

View full text Add to dashboard Cite

Optogenetic tools, providing non‐invasive control over selected cells, have the potential to revolutionize sensory prostheses for humans. Optogenetic stimulation of spiral ganglion neurons (SGNs) in the ear provides a future alternative to electrical stimulation used in cochlear implants. However, most channelrhodopsins do not support the high temporal fidelity pertinent to auditory coding because they require milliseconds to close after light‐off. Here, we biophysically characterized the fast channelrhodopsin Chronos and revealed a deactivation time constant of less than a millisecond at body temperature. In order to enhance neural expression, we improved its trafficking to the plasma membrane (Chronos‐ES/TS). Following efficient transduction of SGNs using early postnatal injection of the adeno‐associated virus AAV‐PHP.B into the mouse cochlea, fiber‐based optical stimulation elicited optical auditory brainstem responses (oABR) with minimal latencies of 1 ms, thresholds of 5 μJ and 100 μs per pulse, and sizable amplitudes even at 1,000 Hz of stimulation. Recordings from single SGNs demonstrated good temporal precision of light‐evoked spiking. In conclusion, efficient virus‐mediated expression of targeting‐optimized Chronos‐ES/TS achieves ultrafast optogenetic control of neurons.

show abstract

Section: Resultscontrasting

confidence: 99%

Ultrafast optogenetic stimulation of the auditory pathway by targeting‐optimized Chronos

et al. 2018

Self Cite

View full text Add to dashboard Cite

show abstract

“…Recent data from conventional synapses suggests that endocytic membrane retrieval per se does not absolutely require AP‐2 or clathrin, which however are both critically required for SV reformation from endosome‐like vacuoles . In line with results obtained in AP‐2μ‐deficient hippocampal neurons, disruption of AP‐2 does not significantly perturb membrane retrieval at IHC ribbon synapses . Upon strong stimulation, loss of AP‐2 leads to the accumulation of endosome‐like vacuoles, which – together with fewer clathrin‐coated pits as well as reduced counts of ribbon‐attached SVs (i.e., at the distal part of the ribbon) – indicates a requirement of AP‐2 for SV reformation.…”

Section: Exocytosis–endocytosis Coupling At Ihc Ribbon Synapsessupporting

confidence: 68%

“…Upon strong stimulation, loss of AP‐2 leads to the accumulation of endosome‐like vacuoles, which – together with fewer clathrin‐coated pits as well as reduced counts of ribbon‐attached SVs (i.e., at the distal part of the ribbon) – indicates a requirement of AP‐2 for SV reformation. Intriguingly, upon prolonged stimulation, the number of membrane‐proximal SVs is unaltered; however, the speed of exocytosis decreases significantly in the mutants, suggesting impaired release site clearance that prevents the membrane‐proximal SVs to reach fusion competence . Otoferlin levels in AP‐2‐deficient IHCs are dramatically reduced and there is an indication that the remaining otoferlin might be more strongly present on the plasma membrane.…”

Section: Exocytosis–endocytosis Coupling At Ihc Ribbon Synapsesmentioning

confidence: 98%

Balancing presynaptic release and endocytic membrane retrieval at hair cell ribbon synapses

Pangršič

Vogl

2018

FEBS Letters

View full text Add to dashboard Cite

The timely and reliable processing of auditory and vestibular information within the inner ear requires highly sophisticated sensory transduction pathways. On a cellular level, these demands are met by hair cells, which respond to sound waves – or alterations in body positioning – by releasing glutamate‐filled synaptic vesicles (SVs) from their presynaptic active zones with unprecedented speed and exquisite temporal fidelity, thereby initiating the auditory and vestibular pathways. In order to achieve this, hair cells have developed anatomical and molecular specializations, such as the characteristic and name‐giving ‘synaptic ribbons’ – presynaptically anchored dense bodies that tether SVs prior to release – as well as other unique or unconventional synaptic proteins. The tightly orchestrated interplay between these molecular components enables not only ultrafast exocytosis, but similarly rapid and efficient compensatory endocytosis. So far, the knowledge of how endocytosis operates at hair cell ribbon synapses is limited. In this Review, we summarize recent advances in our understanding of the SV cycle and molecular anatomy of hair cell ribbon synapses, with a focus on cochlear inner hair cells.

show abstract

“…Furthermore, Peterson et al () found that this model does not readily account for the serial ISI correlations in ANF spontaneous spike trains and their dependence on mean ISI. More recently, Jung et al () suggested that a gamma contribution might arise if two slow transitions, rather than one, existed in the work cycle of a presynaptic vesicle (involving, e.g., vesicle release, release site clearance, and refilling). It is unclear how well such a model can reproduce empirical ISI distributions and whether it accounts for serial ISI correlations and spike‐count statistics, including their dependence on mean ISI.…”

Section: Models Of Anf Spontaneous Activitymentioning

confidence: 99%

Spike timing in auditory‐nerve fibers during spontaneous activity and phase locking

Heil

Peterson

2016

Synapse

View full text Add to dashboard Cite

In vertebrates, all acoustic information transmitted from the inner ear to the central auditory system is relayed by primary auditory afferents (auditory-nerve fibers; ANFs). These neurons are also the most peripheral elements to use action potentials (spikes) to encode the acoustic information. Here, we review what is known about the spiking of ANFs during spontaneous activity, when spike timing might be regarded as largely random, and during stimulation by low-frequency sounds, when spikes are phase locked to the stimulus waveform, a phenomenon generally considered a hallmark of temporal precision and speed in the auditory system. We focus on mammals, in which each ANF is driven by a single ribbon synapse in a single receptor cell, but also cover relevant research on ANFs of vertebrates from other classes. For spontaneous activity, we highlight several spike-history effects in interspike interval distributions, hazard-rate functions, serial interval correlations, and spike-count statistics. We also review models that have attempted to account for these properties. For phase locking, we focus on the responses to low-frequency tones, rather than to low-frequency components of broadband signals such as noise or clicks. We critically review the measures commonly used to quantify phase locking and urge caution when interpreting such measures with respect to spike-timing precision. We also review the dependence of phase locking on stimulus amplitude and frequency. Finally, we identify some open questions.

show abstract

Disruption of adaptor protein 2μ ( AP ‐2μ) in cochlear hair cells impairs vesicle reloading of synaptic release sites and hearing

Cited by 88 publications

References 54 publications

Ultrafast optogenetic stimulation of the auditory pathway by targeting‐optimized Chronos

Ultrafast optogenetic stimulation of the auditory pathway by targeting‐optimized Chronos

Balancing presynaptic release and endocytic membrane retrieval at hair cell ribbon synapses

Spike timing in auditory‐nerve fibers during spontaneous activity and phase locking

Contact Info

Product

Resources

About