Structural features of heteromeric channels composed of CALHM2 and CALHM4 paralogs

  1. Katarzyna Drożdżyk
  2. Martina Peter
  3. Raimund Dutzler

  • Curated by eLife

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    eLife assessment

    In this interesting study, Drożdżyk and colleagues analyze the ability of placental CALHM orthologs to form stable complexes, identifying that CALHM2 and CALHM4 form heterooligomeric channels. The authors then determine cryo-EM structures of heterooligomeric CALHM2 and CALHM4 that reveal a distinct arrangement in which the two orthologs can interact, but preferentially segregate in the channel. This is an important study; the data provide compelling support for the interpretations and overall, the work is clearly described.

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Abstract

The CALHM proteins constitute a family of large pore channels that contains six closely related paralogs in human. Two family members, CALHM1 and 3, have been associated with the release of ATP during taste sensation. Both proteins form heteromeric channels that activate at positive potential and decreased extracellular Ca 2+ concentration. Although the structures of several family members displayed large oligomeric organizations of different size, their function has in most cases remained elusive. Our previous study has identified the paralogs CALHM2, 4 and 6 to be highly expressed in the placenta and defined their structural properties as membrane proteins exhibiting features of large pore channels with unknown activation properties (Drozdzyk et al., 2020). Here we investigated whether these placental paralogs would form heteromers and characterized heteromeric complexes consisting of CALHM2 and CALHM4 subunits using specific binders as fiducial markers. Both proteins assemble with different stoichiometries with the largest population containing CALHM2 as predominant component. In these oligomers, the subunits segregate and reside in their preferred conformation found in homomeric channels. Our study has thus revealed the properties that govern the formation of CALHM heteromers in a process of potential relevance in a cellular context.

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  1. Version published to 10.1101/2024.01.18.576238v3 on bioRxiv
  2. Version published to 10.7554/elife.96138 on eLife
  3. Version published to 10.7554/elife.96138.2 on eLife
  4. eLife

    Author response:

    The following is the authors’ response to the original reviews.

    We thank both reviewers for their supportive comments. Reviewer 1 has suggested a different data processing strategy to better resolve subunits at the CALHM4/CALHM2 interface:

    I recommend an alternative data processing strategy. First, refine particles with 2-4 CALHM4 subunits with symmetry imposed. This is followed by symmetry expansion, signal subtraction of two adjacent subunits, and subsequent classification and refinement of the subtracted particles. This approach, while not guaranteed, can potentially provide a clearer definition of CALHM2 and CALHM4 interfaces and show whether CALHM2 subunits adopt different conformations based on their proximity to CALHM4 subunits.

    We have followed the recommended strategy in an attempt to improve the resolution and better resolve the structural heterogeneity in CALHM2/4 channels. To this end, we have combined symmetry expansion and partial signal subtraction, as suggested by the reviewer. Initially, a symmetrized (C11) 3.4 Å consensus map of undecameric CALHM2/4 channels bound to sybodies SbC2 and SbC4 was used. The particles of this reconstruction were subjected to symmetry expansion (C11) followed by signal subtraction of nine adjacent subunits. Next, we performed focused, alignment-free 3D classification of the remaining two subunits followed by refinement of these classes, leading to the classification of CALHM subunit pairs. The majority of the classes feature well-resolved CALHM2 pairs, consistent with the original approach (Author response image 1A). A minority of the classes contain CALHM4 subunits, revealing heterogeneity similar to regions of CALHM4 subunits observed in the non-symmetrized channel reconstruction (Author response image 1B). Unfortunately, this approach thus did not improve resolution or facilitate a more accurate subunit assignment. Consequently, we decided not to include these attempts in our manuscript. The resubmitted version thus contains only small corrections compared to the previous version.

    Author response image 1.

    Classification of subunit pairs of undecameric CALHM2/4 channels bound to sybodies SbC2 and SbC4 after the processing combining symmetry expansion and partial signal subtraction. (A) Classes showing CALHM2 subunit pairs. (B) Classes showing subunits at interfaces to CALHM4.

  5. eLife

    eLife assessment

    In this interesting study, Drożdżyk and colleagues analyze the ability of placental CALHM orthologs to form stable complexes, identifying that CALHM2 and CALHM4 form heterooligomeric channels. The authors then determine cryo-EM structures of heterooligomeric CALHM2 and CALHM4 that reveal a distinct arrangement in which the two orthologs can interact, but preferentially segregate in the channel. This is an important study; the data provide compelling support for the interpretations and overall, the work is clearly described.

  6. eLife

    Reviewer #1 (Public Review):

    The Calcium Homeostasis Modulators (CALHM) are a family of large pore channels, of which the physiological role of CALHM1 and 3 is well understood, in particular their key role in taste sensation via the release of the neurotransmitter ATP. The activation mechanism of CALHM1 involves membrane depolarization and a decrease in extracellular Ca concentration, allowing the passage of large cellular metabolites. However, the activation mechanism and physiological roles of other family members are much less well understood. Many structures of homomeric CALHM proteins have been determined, revealing distinct oligomeric assemblies despite a common transmembrane domain topology. CALHM1 and 3 have been shown functionally to form heteromeric assemblies with properties distinct from those of homomeric CALHM1. However, the structural basis of heteromeric CALHM1 and 3 remains unexplored.

    In this paper, Drozdzyk et al. present an important study on the structures of heteromeric channels composed of CALHM2 and CALHM4, extending the structural understanding of the CALHM family beyond homomeric channels. The study relies primarily on cryo-EM. Despite the inherent challenges of structural determination due to the similar structural features of CALHM2 and CALHM4, the authors innovatively use synthetic nanobodies to distinguish between the subunits. Their results show a broad distribution of different heteromeric assemblies, with CALHM4 conformation similar to its homomeric form and CALHM2 conformation influenced by its proximity to CALHM4, and provide detailed insights into the interaction between CALHM2 and CALHM4.

    The manuscript is well-structured and presents clear results that support the conclusions drawn. The discovery of heteromeric CALHM channels, although currently limited to an overexpressed system, represents a significant advance in the field of large-pore channels and will certainly encourage further investigation into the physiological relevance and roles of heteromeric CALHM channels.

    Comments on the revised version:

    I appreciate the authors' efforts to try the alternative data processing strategy. Congratulations to the authors for this interesting and important work!

  7. eLife

    Reviewer #2 (Public Review):

    Summary:

    The authors identified that two of the placental CALHM orthologs, CALHM2 and CALHM4 can form heterooligomeric channels that are stable following detergent solubilization. By adding fiducial markers that specifically recognize either CALHM2 or CALHM4, the authors determine a cryo-EM density map of heterooligomeric CALHM2/CALHM4 from which they can determine how the channel in assembled. Surprisingly, the two orthologs segregate into two distinct segments of the channel. This segregation enables the interfacial subunits to ease the transition between the preferred conformations of each ortholog, which are similar to the confirmation that each ortholog adopts in homooligomeric channels.

    Strengths:

    Through the use of fiducial markers, the authors can clearly distinguish between the CALHM2 and CALHM4 promoters in the heterooligomeric channels, strengthening their assignment of most of the promoters. The authors take appropriate caution in identifying two subunits that are likely a mix of the two orthologs in the channel.

    Weaknesses:

    Despite the authors' efforts, no currents could be observed that corresponded to CALHM2/CALHM4 channels and thus the functional effect of their interaction is not known.

  8. Version published to 10.1101/2024.01.18.576238v2 on bioRxiv
  9. Version published to 10.7554/elife.96138.1 on eLife
  10. eLife

    eLife assessment

    In this interesting study, Drożdżyk and colleagues analyze the ability of placental CALHM orthologs to form stable complexes, identifying that CALHM2 and CALHM4 form heterooligomeric channels. The authors then determine cryo-EM structures of heterooligomeric CALHM2 and CALHM4 that reveal a distinct arrangement in which the two orthologs can interact, but preferentially segregate in the channel. This is an important study; the data provide compelling support for the interpretations and overall, the work is clearly described.

  11. eLife

    Reviewer #1 (Public Review):

    The Calcium Homeostasis Modulators (CALHM) are a family of large pore channels, of which the physiological role of CALHM1 and 3 is well understood, in particular their key role in taste sensation via the release of the neurotransmitter ATP. The activation mechanism of CALHM1 involves membrane depolarization and a decrease in extracellular Ca concentration, allowing the passage of large cellular metabolites. However, the activation mechanism and physiological roles of other family members are much less well understood. Many structures of homomeric CALHM proteins have been determined, revealing distinct oligomeric assemblies despite a common transmembrane domain topology. CALHM1 and 3 have been shown functionally to form heteromeric assemblies with properties distinct from those of homomeric CALHM1. However, the structural basis of heteromeric CALHM1 and 3 remains unexplored.

    In this paper, Drozdzyk et al. present an important study on the structures of heteromeric channels composed of CALHM2 and CALHM4, extending the structural understanding of the CALHM family beyond homomeric channels. The study relies primarily on cryo-EM. Despite the inherent challenges of structural determination due to the similar structural features of CALHM2 and CALHM4, the authors innovatively use synthetic nanobodies to distinguish between the subunits. Their results show a broad distribution of different heteromeric assemblies, with CALHM4 conformation similar to its homomeric form and CALHM2 conformation influenced by its proximity to CALHM4, and provide detailed insights into the interaction between CALHM2 and CALHM4.

    The manuscript is well-structured and presents clear results that support the conclusions drawn. The discovery of heteromeric CALHM channels, although currently limited to an overexpressed system, represents a significant advance in the field of large-pore channels and will certainly encourage further investigation into the physiological relevance and roles of heteromeric CALHM channels. The manuscript would benefit from further insight into the functional properties of these heteromeric channels. However, this is not a weakness as the identification of precise activation stimuli for CALHM2 and 4 is beyond the scope of this work.

    A challenge noted is the wide distribution of heteromeric assemblies in the 3D classification, resulting in insufficient particles for high-resolution structure determination of each assembly. The authors choose to combine particles from assemblies with 2-4 copies of CALHM4, which reveals the interface between CALHM2 and 4 but may compromise the quality of structural details. I recommend an alternative data processing strategy. First, refine particles with 2-4 CALHM4 subunits with symmetry imposed. This is followed by symmetry expansion, signal subtraction of two adjacent subunits, and subsequent classification and refinement of the subtracted particles. This approach, while not guaranteed, can potentially provide a clearer definition of CALHM2 and CALHM4 interfaces and show whether CALHM2 subunits adopt different conformations based on their proximity to CALHM4 subunits.

  12. eLife

    Reviewer #2 (Public Review):

    Summary:

    The authors identified that two of the placental CALHM orthologs, CALHM2 and CALHM4 can form heterooligomeric channels that are stable following detergent solubilization. By adding fiducial markers that specifically recognize either CALHM2 or CALHM4, the authors determine a cryo-EM density map of heterooligomeric CALHM2/CALHM4 from which they can determine how the channel is assembled. Surprisingly, the two orthologs segregate into two distinct segments of the channel. This segregation enables the interfacial subunits to ease the transition between the preferred conformations of each ortholog, which are similar to the confirmation that each ortholog adopts in homooligomeric channels.

    Strengths:

    Through the use of fiducial markers, the authors can clearly distinguish between the CALHM2 and CALHM4 promoters in the heterooligomeric channels, strengthening their assignment of most of the promoters. The authors take appropriate caution in identifying two subunits that are likely a mix of the two orthologs in the channel.

    Weaknesses:

    Despite the authors' efforts, no currents could be observed that corresponded to CALHM2/CALHM4 channels and thus the functional effect of their interaction is not known.

  13. Version published to 10.1101/2024.01.18.576238v1 on bioRxiv