Aminosulfonate Modulated pH-induced Conformational Changes in Connexin26 Hemichannels

Yu, Ji Haeng; Bippes, Christian A.; Hand, Galen M.; Müller, Daniel J.; Sosinsky, Gina E.

doi:10.1074/jbc.m609317200

Cited by 75 publications

(68 citation statements)

References 74 publications

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“…Prior to SMFS, membranes containing densely packed SteT were located by contact mode AFM imaging. If necessary, the AFM stylus was used as a nanoscalpel to remove aggregates or the upper layer of the vesicles (47,48). An unperturbed area of the membrane patch was selected, and the AFM stylus was pushed onto the membrane at a force of ϳ750 pN for 0.5-1.0 s to promote unspecific attachment of the SteT polypeptide to the AFM stylus.…”

Section: Methodsmentioning

confidence: 99%

Substrate Binding Tunes Conformational Flexibility and Kinetic Stability of an Amino Acid Antiporter

Bippes

Zeltina

Casagrande

et al. 2009

Journal of Biological Chemistry

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We used single molecule dynamic force spectroscopy to unfold individual serine/threonine antiporters SteT from Bacillus subtilis. The unfolding force patterns revealed interactions and energy barriers that stabilized structural segments of SteT. Substrate binding did not establish strong localized interactions but appeared to be facilitated by the formation of weak interactions with several structural segments. Upon substrate binding, all energy barriers of the antiporter changed thereby describing the transition from brittle mechanical properties of SteT in the unbound state to structurally flexible conformations in the substrate-bound state. The lifetime of the unbound state was much shorter than that of the substrate-bound state. This leads to the conclusion that the unbound state of SteT shows a reduced conformational flexibility to facilitate specific substrate binding and a reduced kinetic stability to enable rapid switching to the bound state. In contrast, the bound state of SteT showed an increased conformational flexibility and kinetic stability such as required to enable transport of substrate across the cell membrane. This result supports the working model of antiporters in which alternate substrate access from one to the other membrane surface occurs in the substrate-bound state.

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Section: Methodsmentioning

confidence: 99%

Substrate Binding Tunes Conformational Flexibility and Kinetic Stability of an Amino Acid Antiporter

Bippes

Zeltina

Casagrande

et al. 2009

Journal of Biological Chemistry

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“…Because biomolecules are 'alive' under these native conditions, AFM has been successfully used to observe single proteins at work; for reviews, see Engel et al (1999) and Engel and Müller (2000). One of the most exciting examples in the literature for the direct visualization of conformational changes is the pH and Ca 2q -dependent opening and closing of the gap junction channel connexin26 Yu et al, 2007). Because of these unique capabilities, AFM is currently being used as a complementary technique to XRC and electron microscopy.…”

Section: Atomic Force Microscopy (Afm)mentioning

confidence: 99%

Structure determination of channel and transport proteins by high-resolution microscopy techniques

Meury

Harder²,

Ucurum³

et al. 2011

Biological Chemistry

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High-resolution microscopy techniques provide a plethora of information on biological structures from the cellular level down to the molecular level. In this review, we present the unique capabilities of transmission electron and atomic force microscopy to assess the structure, oligomeric state, function and dynamics of channel and transport proteins in their native environment, the lipid bilayer. Most importantly, membrane proteins can be visualized in the frozen-hydrated state and in buffer solution by cryo-transmission electron and atomic force microscopy, respectively. We also illustrate the potential of the scintillation proximity assay to study substrate binding of detergent-solubilized transporters prior to crystallization and structural characterization.

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“…KirVac3.1 is one member of a family of transmembrane potassium channels, and gating of Kir channels is spontaneous but modulated by intracellular molecules such as lipids (PIP2), G-proteins, nucleotides, and ions (H + , Ca 2+ , Mg 2+ ). Yu et al (2007) demonstrated that pH-induced conformational changes in connexin 26 hemichannels were modulated by aminosulfonate. They removed the upper layer of the gap junction channel by repetitive scanning AFM tip with loading of strong force.…”

Section: Imaging Of Membrane Channelsmentioning

confidence: 99%

“…Efforts to observe the ultra-structures of cells using AFM have gradually increased since its invention Muller and Engel, 1999;Kreplak et al, 2007;Jaroslawski et al, 2007;Yu et al, 2007). Early studies of cells with AFM were focused on topological observation by high-reso-lution imaging.…”

Section: Applications Of Afm To Imaging Of Membrane Proteinsmentioning

confidence: 99%

“…AFM has been used for the study of membrane channels because it allows observation of cell surfaces in their native environment at remarkable resolution (Jaroslawski et al 2007;Yu et al, 2007;Muller, 2008;Stewart et al, 2010). Jaroslawski et al (2007) have directly visualized gating of KirBac3.1 potassium channels by AFM imaging.…”

Section: Imaging Of Membrane Channelsmentioning

confidence: 99%

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Molecular imaging of membrane proteins and microfilaments using atomic force microscopy

Jung

Park

et al. 2010

Exp Mol Med

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Atomic force microscopy (AFM) is an emerging technique for a variety of uses involving the analysis of cells. AFM is widely applied to obtain information about both cellular structural and subcellular events. In particular, a variety of investigations into membrane proteins and microfilaments were performed with AFM. Here, we introduce applications of AFM to molecular imaging of membrane proteins, and various approaches for observation and identification of intracellular microfilaments at the molecular level. These approaches can contribute to many applications of AFM in cell imaging.

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Aminosulfonate Modulated pH-induced Conformational Changes in Connexin26 Hemichannels

Cited by 75 publications

References 74 publications

Substrate Binding Tunes Conformational Flexibility and Kinetic Stability of an Amino Acid Antiporter

Substrate Binding Tunes Conformational Flexibility and Kinetic Stability of an Amino Acid Antiporter

Structure determination of channel and transport proteins by high-resolution microscopy techniques

Molecular imaging of membrane proteins and microfilaments using atomic force microscopy

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