Your search keyword '"Translocase"' showing total 2,152 results

1. Plant PI4P is required for bacteria to translocate type‐3 effectors.

Author

Peng, Jinfeng, Zhang, Liyuan, Lu, Kai, Chen, Xiaochen, Pang, Hao, Yao, Xiaohui, Li, Ping, Cao, Peng, Li, Xiaoxu, Wang, Zuodong, Qin, Lina, Zhou, Miao, Wang, Maoling, Li, Qizhen, Qiu, Chunyu, Sun, Mingxin, Li, Yufen, Gong, Liping, Wei, Xinlin, and Wang, Siyi

Abstract

Summary Type‐3 effectors (T3E) of phytopathogenic Gram‐negative bacteria fulfill a virulent role, causing disease, or an avirulent role, inducing immunity, following their translocation into plant cells. This study aimed to validate the hypothesis that bacterial T3E translocation requires lipidic compounds in plant cell membranes. Based on genetic, molecular, and biochemical assays, we determined that phosphatidylinositol 4‐phosphate (PI4P) associated with plant cell membranes is essential for the translocation of T3E by bacterial pathogens. Replicate experimental data revealed that PI4P cooperates with the type‐3 translocase HrpF to facilitate the translocation of effectors TAL and Xop from Xanthomonas oryzae and Hop from Pseudomonas syringae into the cells of Oryza sativa and Nicotiana benthamiana, respectively. Genetic and molecular analyses confirmed that, once translocated into plant cells, the distinct effectors induce disease or immunity. Combined genetic and pharmacological analyses revealed that when PI4P content is suppressed via genetic or pharmacological measures, the T3 effector translocation is considerably suppressed, resulting in serious inhibition of bacterial infection. Overall, these findings demonstrate that cooperative functioning of HrpF–PI4P is conserved in bacterial effectors and plants. [ABSTRACT FROM AUTHOR]

Published

2024

2. Host Tropism and Structural Biology of ABC Toxin Complexes.

Author

Martin, Cole L., Hill, John H., and Aller, Stephen G.

Subjects

*BIOPESTICIDES, *VIRAL tropism, *BIOTECHNOLOGY, *X-ray crystallography, *PEPTIDES

Abstract

ABC toxin complexes are a class of protein toxin translocases comprised of a multimeric assembly of protein subunits. Each subunit displays a unique composition, contributing to the formation of a syringe-like nano-machine with natural cargo carrying, targeting, and translocation capabilities. Many of these toxins are insecticidal, drawing increasing interest in agriculture for use as biological pesticides. The A subunit (TcA) is the largest subunit of the complex and contains domains associated with membrane permeation and targeting. The B and C subunits, TcB and TcC, respectively, package into a cocoon-like structure that contains a toxic peptide and are coupled to TcA to form a continuous channel upon final assembly. In this review, we outline the current understanding and gaps in the knowledge pertaining to ABC toxins, highlighting seven published structures of TcAs and how these structures have led to a better understanding of the mechanism of host tropism and toxin translocation. We also highlight similarities and differences between homologues that contribute to variations in host specificity and conformational change. Lastly, we review the biotechnological potential of ABC toxins as both pesticides and cargo-carrying shuttles that enable the transport of peptides into cells. [ABSTRACT FROM AUTHOR]

Published

2024

3. Host Tropism and Structural Biology of ABC Toxin Complexes

Author

Cole L. Martin, John H. Hill, and Stephen G. Aller

Subjects

ABC toxins, translocase, cryo-EM, host tropism, structural biology, X-ray crystallography, Medicine

Abstract

ABC toxin complexes are a class of protein toxin translocases comprised of a multimeric assembly of protein subunits. Each subunit displays a unique composition, contributing to the formation of a syringe-like nano-machine with natural cargo carrying, targeting, and translocation capabilities. Many of these toxins are insecticidal, drawing increasing interest in agriculture for use as biological pesticides. The A subunit (TcA) is the largest subunit of the complex and contains domains associated with membrane permeation and targeting. The B and C subunits, TcB and TcC, respectively, package into a cocoon-like structure that contains a toxic peptide and are coupled to TcA to form a continuous channel upon final assembly. In this review, we outline the current understanding and gaps in the knowledge pertaining to ABC toxins, highlighting seven published structures of TcAs and how these structures have led to a better understanding of the mechanism of host tropism and toxin translocation. We also highlight similarities and differences between homologues that contribute to variations in host specificity and conformational change. Lastly, we review the biotechnological potential of ABC toxins as both pesticides and cargo-carrying shuttles that enable the transport of peptides into cells.

Published

2024

4. Unique Interactions of the Small Translocases of the Mitochondrial Inner Membrane (Tims) in Trypanosoma brucei.

Author

Quiñones, Linda S., Gonzalez, Fidel Soto, Darden, Chauncey, Khan, Muhammad, Tripathi, Anuj, Smith Jr., Joseph T., Davis, Jamaine, Misra, Smita, and Chaudhuri, Minu

Subjects

*TRYPANOSOMA brucei, *MITOCHONDRIAL membranes, *GEL permeation chromatography, *AFRICAN trypanosomiasis, *TRYPANOSOMA

Abstract

The infectious agent for African trypanosomiasis, Trypanosoma brucei, possesses a unique and essential translocase of the mitochondrial inner membrane, known as the TbTIM17 complex. TbTim17 associates with six small TbTims (TbTim9, TbTim10, TbTim11, TbTim12, TbTim13, and TbTim8/13). However, the interaction patterns of these smaller TbTims with each other and TbTim17 are not clear. Through yeast two-hybrid (Y2H) and co-immunoprecipitation analyses, we demonstrate that all six small TbTims interact with each other. Stronger interactions were found among TbTim8/13, TbTim9, and TbTim10. However, TbTim10 shows weaker associations with TbTim13, which has a stronger connection with TbTim17. Each of the small TbTims also interacts strongly with the C-terminal region of TbTim17. RNAi studies indicated that among all small TbTims, TbTim13 is most crucial for maintaining the steady-state levels of the TbTIM17 complex. Further analysis of the small TbTim complexes by size exclusion chromatography revealed that each small TbTim, except for TbTim13, is present in ~70 kDa complexes, possibly existing in heterohexameric forms. In contrast, TbTim13 is primarily present in the larger complex (>800 kDa) and co-fractionates with TbTim17. Altogether, our results demonstrate that, relative to other eukaryotes, the architecture and function of the small TbTim complexes are specific to T. brucei. [ABSTRACT FROM AUTHOR]

Published

2024

5. Envisioning how the prototypic molecular machine TFIIH functions in transcription initiation and DNA repair

Author

Tsutakawa, Susan E, Tsai, Chi-Lin, Yan, Chunli, Bralić, Amer, Chazin, Walter J, Hamdan, Samir M, Schärer, Orlando D, Ivanov, Ivaylo, and Tainer, John A

Subjects

Genetics, 2.1 Biological and endogenous factors, Aetiology, 1.1 Normal biological development and functioning, Underpinning research, Cancer, Generic health relevance, Good Health and Well Being, DNA, DNA Damage, DNA Helicases, DNA Repair, DNA-Binding Proteins, Humans, Models, Molecular, Protein Conformation, Transcription Factor TFIIH, Transcription Initiation, Genetic, Xeroderma Pigmentosum Group D Protein, TFIIH, Helicase, Transcription initiation, Transcription-coupled repair, Nucleotide excision repair, XPB, XPD, Translocase, DNA damage, DNA repair, Biochemistry and Cell Biology, Developmental Biology

Abstract

Critical for transcription initiation and bulky lesion DNA repair, TFIIH provides an exemplary system to connect molecular mechanisms to biological outcomes due to its strong genetic links to different specific human diseases. Recent advances in structural and computational biology provide a unique opportunity to re-examine biologically relevant molecular structures and develop possible mechanistic insights for the large dynamic TFIIH complex. TFIIH presents many puzzles involving how its two SF2 helicase family enzymes, XPB and XPD, function in transcription initiation and repair: how do they initiate transcription, detect and verify DNA damage, select the damaged strand for incision, coordinate repair with transcription and cell cycle through Cdk-activating-kinase (CAK) signaling, and result in very different specific human diseases associated with cancer, aging, and development from single missense mutations? By joining analyses of breakthrough cryo-electron microscopy (cryo-EM) structures and advanced computation with data from biochemistry and human genetics, we develop unified concepts and molecular level understanding for TFIIH functions with a focus on structural mechanisms. We provocatively consider that TFIIH may have first evolved from evolutionary pressure for TCR to resolve arrested transcription blocks to DNA replication and later added its key roles in transcription initiation and global DNA repair. We anticipate that this level of mechanistic information will have significant impact on thinking about TFIIH, laying a robust foundation suitable to develop new paradigms for DNA transcription initiation and repair along with insights into disease prevention, susceptibility, diagnosis and interventions.

Published

2020

6. Mycobacterial type VII secretion systems.

Author

Famelis, Nikolaos, Geibel, Sebastian, and van Tol, Daan

Subjects

*CARRIER proteins, *PROTEIN transport, *BACTERIAL cell surfaces, *SECRETION, *TUBERCULOSIS, *MYCOBACTERIA

Abstract

Mycobacteria, such as the pathogen M. tuberculosis, utilize up to five paralogous type VII secretion systems to transport proteins across their cell envelope. Since these proteins associate in pairs that depend on each other for transport to a different extent, the secretion pathway to the bacterial surface remained challenging to address. Structural characterization of the inner-membrane embedded secretion machineries along with recent advances on the substrates' co-dependencies for transport allow for the first time more detailed and testable models for secretion. [ABSTRACT FROM AUTHOR]

Published

2023

7. Structural and DNA end resection study of the bacterial NurA-HerA complex

Author

Jieyu Yang, Yiyang Sun, Ying Wang, Wanshan Hao, and Kaiying Cheng

Subjects

Deinococcus, DNA end resection, Nuclease, NurA-HerA, Translocase, Biology (General), QH301-705.5

Abstract

Abstract Background The nuclease NurA and the ATPase/translocase HerA play a vital role in repair of double-strand breaks (DSB) during the homologous recombination in archaea. A NurA-HerA complex is known to mediate DSB DNA end resection, leading to formation of a free 3′ end used to search for the homologous sequence. Despite the structures of individual archaeal types of NurA and HerA having been reported, there is limited information regarding the molecular mechanisms underlying this process. Some bacteria also possess homologs of NurA and HerA; however, the bacterial type of this complex, as well as the detailed mechanisms underlying the joining of NurA-HerA in DSB DNA end resection, remains unclear. Results We report for the first time the crystal structures of Deinococcus radiodurans HerA (drHerA) in the nucleotide-free and ADP-binding modes. A D. radiodurans NurA-HerA complex structure was constructed according to a low-resolution cryo-electron microscopy map. We performed site-directed mutagenesis to map the drNurA-HerA interaction sites, suggesting that their interaction is mainly mediated by ionic links, in contrast to previously characterized archaeal NurA-HerA interactions. The key residues responsible for the DNA translocation activity, DNA unwinding activity, and catalytic activities of the drNurA-HerA complex were identified. A HerA/FtsK-specific translocation-related motif (TR motif) that guarantees the processivity of double-stranded DNA (dsDNA) translocation was identified. Moreover, a mechanism for the translocation-regulated resection of the 5′ tail of broken dsDNA and the corresponding generation of a recombinogenic 3′ single-stranded DNA tail by the drNurA-HerA complex was elucidated. Conclusions Our work provides new insights into the mechanism underlying bacterial NurA-HerA-mediated DSB DNA end resection, and the way this complex digests the 5′ tail of a DNA duplex and provides long 3′ free end for strand invasion in the bacterial homologous recombination process.

Published

2023

8. Structural and DNA end resection study of the bacterial NurA-HerA complex.

Author

Yang, Jieyu, Sun, Yiyang, Wang, Ying, Hao, Wanshan, and Cheng, Kaiying

Subjects

*DNA, *DEINOCOCCUS radiodurans, *SITE-specific mutagenesis, *DNA denaturation, *SINGLE-stranded DNA, *CATALYTIC activity

Abstract

Background: The nuclease NurA and the ATPase/translocase HerA play a vital role in repair of double-strand breaks (DSB) during the homologous recombination in archaea. A NurA-HerA complex is known to mediate DSB DNA end resection, leading to formation of a free 3′ end used to search for the homologous sequence. Despite the structures of individual archaeal types of NurA and HerA having been reported, there is limited information regarding the molecular mechanisms underlying this process. Some bacteria also possess homologs of NurA and HerA; however, the bacterial type of this complex, as well as the detailed mechanisms underlying the joining of NurA-HerA in DSB DNA end resection, remains unclear. Results: We report for the first time the crystal structures of Deinococcus radiodurans HerA (drHerA) in the nucleotide-free and ADP-binding modes. A D. radiodurans NurA-HerA complex structure was constructed according to a low-resolution cryo-electron microscopy map. We performed site-directed mutagenesis to map the drNurA-HerA interaction sites, suggesting that their interaction is mainly mediated by ionic links, in contrast to previously characterized archaeal NurA-HerA interactions. The key residues responsible for the DNA translocation activity, DNA unwinding activity, and catalytic activities of the drNurA-HerA complex were identified. A HerA/FtsK-specific translocation-related motif (TR motif) that guarantees the processivity of double-stranded DNA (dsDNA) translocation was identified. Moreover, a mechanism for the translocation-regulated resection of the 5′ tail of broken dsDNA and the corresponding generation of a recombinogenic 3′ single-stranded DNA tail by the drNurA-HerA complex was elucidated. Conclusions: Our work provides new insights into the mechanism underlying bacterial NurA-HerA-mediated DSB DNA end resection, and the way this complex digests the 5′ tail of a DNA duplex and provides long 3′ free end for strand invasion in the bacterial homologous recombination process. [ABSTRACT FROM AUTHOR]

Published

2023

9. A hypomorphic variant in the translocase of the outer mitochondrial membrane complex subunit TOMM7 causes short stature and developmental delay

Author

Cameron Young, Dominyka Batkovskyte, Miyuki Kitamura, Maria Shvedova, Yutaro Mihara, Jun Akiba, Wen Zhou, Anna Hammarsjö, Gen Nishimura, Shuichi Yatsuga, Giedre Grigelioniene, and Tatsuya Kobayashi

Subjects

mitochondria, TOM, translocase, TOMM7, skeletal dysplasia, lipoatrophy, Genetics, QH426-470

Abstract

Summary: Mitochondrial diseases are a heterogeneous group of genetic disorders caused by pathogenic variants in genes encoding gene products that regulate mitochondrial function. These genes are located either in the mitochondrial or in the nuclear genome. The TOMM7 gene encodes a regulatory subunit of the translocase of outer mitochondrial membrane (TOM) complex that plays an essential role in translocation of nuclear-encoded mitochondrial proteins into mitochondria. We report an individual with a homozygous variant in TOMM7 (c.73T>C, p.Trp25Arg) that presented with a syndromic short stature, skeletal abnormalities, muscle hypotonia, microvesicular liver steatosis, and developmental delay. Analysis of mouse models strongly suggested that the identified variant is hypomorphic because mice homozygous for this variant showed a milder phenotype than those with homozygous Tomm7 deletion. These Tomm7 mutant mice show pathological changes consistent with mitochondrial dysfunction, including growth defects, severe lipoatrophy, and lipid accumulation in the liver. These mice die prematurely following a rapidly progressive weight loss during the last week of their lives. Tomm7 deficiency causes a unique alteration in mitochondrial function; despite the bioenergetic deficiency, mutant cells show increased oxygen consumption with normal responses to electron transport chain (ETC) inhibitors, suggesting that Tomm7 deficiency leads to an uncoupling between oxidation and ATP synthesis without impairing the function of the tricarboxylic cycle metabolism or ETC. This study presents evidence that a hypomorphic variant in one of the genes encoding a subunit of the TOM complex causes mitochondrial disease.

Published

2023

10. The natural bicyclic hexapeptide RA-VII is a novel inhibitor of the eukaryotic translocase eEF2.

Author

Miyoshi, Tomohiro, Nomura, Takaomi, Takeya, Koich, and Uchiumi, Toshio

Subjects

*HEXAPEPTIDES, *BINDING site assay, *PROTEIN synthesis, *EUKARYOTIC cells, *GUANOSINE triphosphatase, *TRANSFER RNA

Abstract

A cyclic hexapeptide, RA-VII isolated from the Rubiaceae family of plants, has high cytotoxic activity. Although RA-VII has been shown to inhibit protein synthesis in eukaryotic cells, the molecular mode of its action is not clear. Here we investigate the mechanism of the RAVII action on the translation apparatus. Biochemical functional assays showed that RA-VII inhibits poly(U)-dependent polyphenylalanine synthesis in the presence of animal elongation factors eEF1A and eEF2. Furthermore, RAVII prevented eEF2/ribosome-dependent GTPase activity, but not eEF-1A/ribosome-dependent activity. A filter binding assay demonstrated that RA-VII markedly enhances the binding affinity of eEF2 for GTP, but not for GDP, and prevents exchange of GTP in the eEF2-GTP complex, even after addition of a large excess of GTP/GDP. Limited proteolysis experiments indicated that RA-VII prevents the digestion of eEF2 in the presence of either GTP or GMPPCP, but not with GDP. Further footprint analysis and a translocation assay showed that the eEF2•GMPPNP•RA-VII complex binds to the conserved rRNA regions at the factor-binding center of the ribosome and retains the ability to translocate the A site-bound tRNA to the P-site. These results suggest that RA-VII tightly stabilizes the GTP•eEF2 complex structure, which is able to bind to the ribosomal functional site, but seems to suppress normal turnover of eEF2 after translocation. The properties of RA-VII make it a novel ligand for probing the action of eEF2 in the process of translocation on the ribosome. [Display omitted] • A cyclic hexapeptide, RA-VII inhibits translation elongation. • RA-VII inhibits eEF2/ribosome-dependent GTPase turnover. • RA-VII tightly stabilizes an eEF2.•GTP complex structure. • RA-VII-stabilized eEF2.•GTP retains ability to bind to the ribosomal functional site. • RA-VII seems to stall eEF2 on the ribosome. [ABSTRACT FROM AUTHOR]

Published

2022

11. New Obstructive Sleep Apnea Data Have Been Reported by Investigators at University of Hong Kong (The Effects of Intermittent Hypoxia On Hepatic Expression of Fatty Acid Translocase Cd36 In Lean and Diet-induced Obese Mice).

Published

2024

12. FANCM branchpoint translocase: Master of traverse, reverse and adverse DNA repair.

Author

Abbouche, Lara, Bythell-Douglas, Rohan, and Deans, Andrew J.

Subjects

*DNA ligases, *DNA repair, *FANCONI'S anemia, *DNA structure, CANCER susceptibility

Abstract

FANCM is a multifunctional DNA repair enzyme that acts as a sensor and coordinator of replication stress responses, especially interstrand crosslink (ICL) repair mediated by the Fanconi anaemia (FA) pathway. Its specialised ability to bind and remodel branched DNA structures enables diverse genome maintenance activities. Through ATP-powered "branchpoint translocation", FANCM can promote fork reversal, facilitate replication traverse of ICLs, resolve deleterious R-loop structures, and restrain recombination. These remodelling functions also support a role as sensor of perturbed replication, eliciting checkpoint signalling and recruitment of downstream repair factors like the Fanconi anaemia FANCI:FANCD2 complex. Accordingly, FANCM deficiency causes chromosome fragility and cancer susceptibility. Other recent advances link FANCM to roles in gene editing efficiency and meiotic recombination, along with emerging synthetic lethal relationships, and targeting opportunities in ALT-positive cancers. Here we review key properties of FANCM's biochemical activities, with a particular focus on branchpoint translocation as a distinguishing characteristic. • FANCM is a DNA repair enzyme that resolves branched DNA structures. • ATP-powered branchpoint translocation enables fork reversal and crosslink traverse. • FANCM also restrains recombination and elicits checkpoint signaling. • FANCM deficiency causes fragile chromosomes, ICL sensitivity and cancer susceptibility. [ABSTRACT FROM AUTHOR]

Published

2024

13. Unsaturated fatty acids augment protein transport via the SecA:SecYEG translocon.

Author

Kamel, Michael, Löwe, Maryna, Schott‐Verdugo, Stephan, Gohlke, Holger, and Kedrov, Alexej

Subjects

*FATTY acid-binding proteins, *UNSATURATED fatty acids, *MOLECULAR dynamics, *BACTERIAL proteins, *IONIC strength

Abstract

The translocon SecYEG and the associated ATPase SecA form the primary protein secretion system in the cytoplasmic membrane of bacteria. The secretion is essentially dependent on the surrounding lipids, but the mechanistic understanding of their role in SecA : SecYEG activity is sparse. Here, we reveal that the unsaturated fatty acids (UFAs) of the membrane phospholipids, including tetraoleoyl‐cardiolipin, stimulate SecA : SecYEG‐mediated protein translocation up to ten‐fold. Biophysical analysis and molecular dynamics simulations show that UFAs increase the area per lipid and cause loose packing of lipid head groups, where the N‐terminal amphipathic helix of SecA docks. While UFAs do not affect the translocon folding, they promote SecA binding to the membrane, and the effect is enhanced up to fivefold at elevated ionic strength. Tight SecA : lipid interactions convert into the augmented translocation. Our results identify the fatty acid structure as a notable factor in SecA : SecYEG activity, which may be crucial for protein secretion in bacteria, which actively change their membrane composition in response to their habitat. [ABSTRACT FROM AUTHOR]

Published

2022

14. Helical inchworming: a novel translocation mechanism for a ring ATPase.

Author

Tong, Alexander B. and Bustamante, Carlos

Abstract

Ring ATPases perform a variety of tasks in the cell. Their function involves complex communication and coordination among the often identical subunits. Translocases in this group are of particular interest as they involve both chemical and mechanical actions in their operation. We study the DNA packaging motor of bacteriophage φ29, and using single-molecule optical tweezers and single-particle cryo-electron microscopy, have discovered a novel translocation mechanism for a molecular motor. [ABSTRACT FROM AUTHOR]

Published

2021

15. Structural basis of elongation factor 2 switching

Author

Michael K. Fenwick and Steven E. Ealick

Subjects

Translation, Elongation factor, Translocase, Translocation, Ribosome, GTPase, Biology (General), QH301-705.5

Abstract

Archaebacterial and eukaryotic elongation factor 2 (EF-2) and bacterial elongation factor G (EF-G) are five domain GTPases that catalyze the ribosomal translocation of tRNA and mRNA. In the classical mechanism of activation, GTPases are switched on through GDP/GTP exchange, which is accompanied by the ordering of two flexible segments called switch I and II. However, crystal structures of EF-2 and EF-G have thus far not revealed the conformations required by the classical mechanism. Here, we describe crystal structures of Methanoperedens nitroreducens EF-2 (MnEF-2) and MnEF-2-H595N bound to GMPPCP (GppCp) and magnesium displaying previously unreported compact conformations. Domain III forms interfaces with the other four domains and the overall conformations resemble that of SNU114, the eukaryotic spliceosomal GTPase. The gamma phosphate of GMPPCP is detected through interactions with switch I and a P-loop structural element. Switch II is highly ordered whereas switch I shows a variable degree of ordering. The ordered state results in a tight interdomain arrangement of domains I-III and the formation of a portion of a predicted monovalent cation site involving the P-loop and switch I. The side chain of an essential histidine residue in switch II is placed in the inactive conformation observed for the “on” state of elongation factor EF-Tu. The compact conformations of MnEF-2 and MnEF-2-H595N suggest an “on” ribosome-free conformational state.

Published

2020

16. Preproteins couple the intrinsic dynamics of SecA to its ATPase cycle to translocate via a catch and release mechanism

Author

Srinath Krishnamurthy, Marios-Frantzeskos Sardis, Nikolaos Eleftheriadis, Katerina E. Chatzi, Jochem H. Smit, Konstantina Karathanou, Giorgos Gouridis, Athina G. Portaliou, Ana-Nicoleta Bondar, Spyridoula Karamanou, and Anastassios Economou

Subjects

translocase, protein secretion, SecA, SecYEG channel, HDX-MS, smFRET, Biology (General), QH301-705.5

Abstract

Summary: Protein machines undergo conformational motions to interact with and manipulate polymeric substrates. The Sec translocase promiscuously recognizes, becomes activated, and secretes >500 non-folded preprotein clients across bacterial cytoplasmic membranes. Here, we reveal that the intrinsic dynamics of the translocase ATPase, SecA, and of preproteins combine to achieve translocation. SecA possesses an intrinsically dynamic preprotein clamp attached to an equally dynamic ATPase motor. Alternating motor conformations are finely controlled by the γ-phosphate of ATP, while ADP causes motor stalling, independently of clamp motions. Functional preproteins physically bridge these independent dynamics. Their signal peptides promote clamp closing; their mature domain overcomes the rate-limiting ADP release. While repeated ATP cycles shift the motor between unique states, multiple conformationally frustrated prongs in the clamp repeatedly “catch and release” trapped preprotein segments until translocation completion. This universal mechanism allows any preprotein to promiscuously recognize the translocase, usurp its intrinsic dynamics, and become secreted.

Published

2022

17. Mapping of a N-terminal α-helix domain required for human PINK1 stabilization, Serine228 autophosphorylation and activation in cells

Author

Poonam Kakade, Hina Ojha, Olawale G. Raimi, Andrew Shaw, Andrew D. Waddell, James R. Ault, Sophie Burel, Kathrin Brockmann, Atul Kumar, Mohd Syed Ahangar, Ewelina M. Krysztofinska, Thomas Macartney, Richard Bayliss, Julia C. Fitzgerald, and Miratul M. K. Muqit

Subjects

PINK1, kinase, mitochondria, translocase, phosphorylation, Parkinson's disease, Biology (General), QH301-705.5

Abstract

Autosomal recessive mutations in the PINK1 gene are causal for Parkinson's disease (PD). PINK1 encodes a mitochondrial localized protein kinase that is a master-regulator of mitochondrial quality control pathways. Structural studies to date have elaborated the mechanism of how mutations located within the kinase domain disrupt PINK1 function; however, the molecular mechanism of PINK1 mutations located upstream and downstream of the kinase domain is unknown. We have employed mutagenesis studies to define the minimal region of human PINK1 required for optimal ubiquitin phosphorylation, beginning at residue Ile111. Inspection of the AlphaFold human PINK1 structure model predicts a conserved N-terminal α-helical extension (NTE) domain forming an intramolecular interaction with the C-terminal extension (CTE), which we corroborate using hydrogen/deuterium exchange mass spectrometry of recombinant insect PINK1 protein. Cell-based analysis of human PINK1 reveals that PD-associated mutations (e.g. Q126P), located within the NTE : CTE interface, markedly inhibit stabilization of PINK1; autophosphorylation at Serine228 (Ser228) and Ubiquitin Serine65 (Ser65) phosphorylation. Furthermore, we provide evidence that NTE and CTE domain mutants disrupt PINK1 stabilization at the mitochondrial Translocase of outer membrane complex. The clinical relevance of our findings is supported by the demonstration of defective stabilization and activation of endogenous PINK1 in human fibroblasts of a patient with early-onset PD due to homozygous PINK1 Q126P mutations. Overall, we define a functional role of the NTE : CTE interface towards PINK1 stabilization and activation and show that loss of NTE : CTE interactions is a major mechanism of PINK1-associated mutations linked to PD.

Published

2022

18. Probing the organisation of the TatC component in the Tat system of Escherichia coli

Author

Cléon, François and Palmer, Tracy

Subjects

579, Twin-arginine, Translocase, Tat, Molecular, Microbiology, Escherichia coli, Membrane, Transport

Abstract

The Tat protein export system transports folded proteins across the bacterial cytoplasmic membrane and the plant thylakoid membrane. In Escherichia coli, the Tat system is composed of the TatA, TatB and TatC proteins. TatB and TatC assemble into a multimeric receptor complex that recognises and binds the substrate, before the TatA protomers cluster at the TatBC complex to facilitate substrate transport. A genetic screen was devised to explore the oligomeric state of TatC, reasoning that the isolation of dominant negative TatC variants that inactivate the Tat system in the presence of a functional copy of wild type TatC would provide strong evidence TatC is an obligate oligomer. Single dominant negative TatC substitutions were isolated that were located in the first and second periplasmic loops of TatC. These substitutions did not prevent TatC from interacting with TatB, TatA, itself or with a Tat substrate. Blue Native PAGE analysis showed that the TatC variants were unable to form the 440 kDa TatBC complex. Surprisingly, the substitutions did not prevent TatC:TatC self-interactions in the periplasmic regions, detected by disulphide cross-linking, but they did abolish a substrate-induced interaction at the fifth transmembrane helix of TatC. Fluorescence microscopy experiments revealed that the dominant negative TatC variants prevented the polymerisation of TatA-YFP in vivo. These results show that TatC possesses at least two interaction interfaces and imply that the periplasmic loops are critical for the transition between substrate binding and TatA polymerisation. Accessibility of single cysteine substitutions in TatC was probed by PEG-Mal labelling in intact cells. TatB was shown to be important for the proper insertion of TatC into the membrane. The absence of TatA led to accessibility changes in the vicinity of the fifth transmembrane domain of TatC, where both TatA and TatB are known to dock. This suggests that TatA and TatB may share an overlapping binding site.

Published

2015

19. Recent Findings from Harbin Medical University Has Provided New Information about Polycystic Ovary Syndrome (translocase of Outer Mitochondrial Membrane 40, As a Promising Biomarker for the Diagnosis of Polycystic Ovary Syndrome and...).

Abstract

A recent study conducted by Harbin Medical University in China has found a potential biomarker for the diagnosis of polycystic ovary syndrome (PCOS) and pan-cancer. The study identified a significant association between translocase of outer mitochondrial membrane 40 (TOMM40) and both PCOS and pan-cancers. TOMM40 was found to be significantly decreased in the PCOS group, and its over-expression was able to rescue the effects induced by DHEA in KGN cells. The research suggests that TOMM40 could be a promising biomarker for diagnosing both PCOS and pan-cancer. [Extracted from the article]

Published

2024

20. University of Paris Researchers Have Published New Study Findings on Lung Cancer (Glucose metabolism transcriptome clustering identifies subsets of resectable lung adenocarcinoma with different prognosesCentral MessagePerspective).

Abstract

A new study conducted by researchers at the University of Paris has identified distinct clusters of glucose metabolism in resectable lung adenocarcinoma, providing valuable prognostic information. The study analyzed RNA expressions from 489 primary lung adenocarcinoma samples and found that higher expression of monocarboxylate transporter 4 (MCT4) was associated with a worse prognosis, while increased expression of translocase of outer mitochondrial membrane 20 (TOMM20) and MCT1 were associated with better outcomes. The study also identified three major metabolic phenotypes with significantly different pathologic stage distribution and prognosis. The findings suggest that considering metabolic profiles could be important in designing strategies for reprogramming energy metabolism in lung cancer treatment. Further research is needed to validate these findings in different cancer types and populations. [Extracted from the article]

Published

2024

21. Adenine nucleotide translocase 2 silencing promotes metabolic adaptations and anoikis in P19 embryonal carcinoma stem cells.

Abstract

A preprint abstract from biorxiv.org discusses the role of adenine nucleotide translocase 2 (ANT2) in cancer stem cells (CSCs). The study focuses on P19 embryonal carcinoma stem cells (P19SCs) as a model for CSCs and uses siRNA to inhibit ANT2 translation. The results show that ANT2 depletion leads to compromised OXPHOS machinery and mitochondrial membrane potential, as well as a metabolic adaptation towards a less oxidative phenotype. The study suggests that ANT2 may be a potential therapeutic target for controlling CSC-driven tumor progression. However, it is important to note that this preprint has not been peer-reviewed. [Extracted from the article]

Published

2024

22. Mechanism of structure-specific DNA binding by the FANCM branchpoint translocase.

Abstract

According to a preprint abstract from biorxiv.org, researchers have discovered that the N-terminal translocase domain of the FANCM protein is responsible for recognizing branched DNA structures. This domain is crucial for effective substrate engagement and DNA binding, as well as for catalytic ATP-dependent branch migration. Mutations in key DNA-binding residues within this domain diminish FANCM's affinity for junction DNA and abolish branch migration activity. These findings suggest that the Hel2i domain plays an essential role in FANCM's tumor-suppressive functions by restraining the hyperactivation of the Alternative Lengthening of Telomeres (ALT) pathway. However, it is important to note that this preprint has not yet been peer-reviewed. [Extracted from the article]

Published

2024

23. Dexamethasone upregulates mitochondrial Tom20, Tom70, and MnSOD through SGK1 in the kidney cells.

Author

Hira, Sharanpreet, Packialakshmi, Balamurugan, Tang, Esther, and Zhou, Xiaoming

Abstract

Dexamethasone augments mitochondrial protein abundance. The translocase of the outer membrane (Tom) of mitochondria plays a major role in importing largely cytosolically synthesized proteins into mitochondria. We hypothesize that dexamethasone upregulates the Tom transport system, leading to increase of mitochondrial protein localization. Tom20 and Tom70 are the two major subunits. Dexamethasone increased Tom20 and Tom70 mRNA levels by 53 ± 11% and 25 ± 9% and mitochondrial protein abundance by 27 ± 7% and 25 ± 4% (p < 0.05 for all), respectively, in HEK293 cells. In parallel, dexamethasone elevated the SGK1 mRNA by 79 ± 17% and activity by 190 ± 42%, and mitochondrial protein level by 41 ± 2% (all p < 0.05) without significantly affecting the cytosol counterpart. The discovery of the effect of dexamethasone on SGK1 protein restricted in the mitochondria attracted us to examine the effect of the hormone on MnSOD, an enzyme with known mitochondrial localization and function. Similarly, dexamethasone significantly increased MnSOD transcripts by 67 ± 15% and protein level only in the mitochondria dose-dependently. Inhibition of SGK1 by GSK650394 and RNAi significantly attenuated the effects of the hormone on Tom20, Tom70, and MnSOD, indicating that SGK1 relays the effects of dexamethasone. Catalase inhibited the effects of dexamethasone on SGK1 and the subsequent effects of SGK1 on Tom20, Tom70, and MnSOD. Finally, knock-down of Tom20 and Tom70 by their siRNAs reduced dexamethasone-induced increases in the mitochondrial localization of SGK1 and MnSOD proteins. In conclusion, dexamethasone upregulates Tom20, Tom70, and MnSOD, and these effects are dependent on reactive oxygen species and SGK1. Dexamethasone-induced increases of SGK1 and MnSOD mitochondrial localization requires Tom20 and Tom70. [ABSTRACT FROM AUTHOR]

Published

2021

24. Novel IM‐associated protein Tim54 plays a role in the mitochondrial import of internal signal‐containing proteins in Trypanosoma brucei.

Author

Singha, Ujjal K., Tripathi, Anuj, Smith, Joseph T., Quinones, Linda, Saha, Aparajita, Singha, Tanusree, and Chaudhuri, Minu

Subjects

*TRYPANOSOMA brucei, *CARRIER proteins, *MITOCHONDRIAL proteins, *AFRICAN trypanosomiasis, *MITOCHONDRIA, *CYTOCHROME oxidase, *TRYPANOSOMA

Abstract

Background: The translocase of the mitochondrial inner membrane (TIM) imports most of the nucleus‐encoded proteins that are destined for the matrix, inner membrane (IM) and the intermembrane space (IMS). Trypanosoma brucei, the infectious agent for African trypanosomiasis, possesses a unique TIM complex consisting of several novel proteins in association with a relatively conserved protein TbTim17. Tandem affinity purification of the TbTim17 protein complex revealed TbTim54 as a potential component of this complex. Results: TbTim54, a trypanosome‐specific IMS protein, is peripherally associated with the IM and is present in a protein complex slightly larger than the TbTim17 complex. TbTim54 knockdown (KD) reduced the import of TbTim17 and compromised the integrity of the TbTim17 complex. TbTim54 KD inhibited the in vitro mitochondrial import and assembly of the internal signal‐containing mitochondrial carrier proteins MCP3, MCP5 and MCP11 to a greater extent than TbTim17 KD. Furthermore, TbTim54 KD, but not TbTim17 KD, significantly hampered the mitochondrial targeting of ectopically expressed MCP3 and MCP11. These observations along with our previous finding that the mitochondrial import of N‐terminal signal‐containing proteins like cytochrome oxidase subunit 4 and MRP2 was affected to a greater extent by TbTim17 KD than TbTim54 KD indicating a substrate‐specificity of TbTim54 for internal‐signal containing mitochondrial proteins. In other organisms, small Tim chaperones in the IMS are known to participate in the translocation of MCPs. We found that TbTim54 can directly interact with at least two of the six known small TbTim proteins, TbTim11 and TbTim13, as well as with the N‐terminal domain of TbTim17. Conclusion: TbTim54 interacts with TbTim17. It also plays a crucial role in the mitochondrial import and complex assembly of internal signal‐containing IM proteins in T. brucei. Significance: We are the first to characterise TbTim54, a novel TbTim that is involved primarily in the mitochondrial import of MCPs and TbTim17 in T. brucei. [ABSTRACT FROM AUTHOR]

Published

2021

25. Structure-function studies of the bacterial dsDNA translocase FtsK

Author

Graham, James Edward, Sherratt, David John, and Turberfield, Andrew J.

Subjects

572.85, Molecular biophysics (biochemistry), Escherichia coli, helicase, translocase, triplex displacement, biophysics, structural biology, chromosome segregation

Abstract

DNA translocases are molecular motors that use energy from nucleotide triphosphate (NTP) hydrolysis to move along, pump, remodel or clear DNA. Unlike helicases, double-stranded DNA (dsDNA) translocases do not unwind DNA; their action has no net product apart from inducing supercoils as a result of groove-tracking, which has hampered their characterisation. Many dsDNA translocases appear to have biased directionality. However, the inherent symmetry of dsDNA requires that translocase activity is regulated by specific sequences or through modulation by interaction partners. FtsK is a highly conserved bacterial cell-division protein, localised to the dividing septum, that coordinates chromosome segregation with cytokinesis. It is responsible for the resolution of chromosome dimers by activating the tyrosine recombinases XerCD bound to the 28bp chromosomal site dif. The C-terminal domain of FtsK (FtsKC) is a dsDNA translocase (speed ~5 kb/s, stall force ~60 pN) most closely related to superfamily 4 helicases and is active as a hexameric ring. A winged-helix subdomain at the C-terminus of FtsKC, FtsKgamma, binds to specific 8 bp sequences, KOPS, that are polarised in the bacterial chromosome from the origin to towards dif. FtsKgamma also interacts with XerD, activating it for catalysis. Studies of FtsK translocation have differed over whether KOPS act as a loading or a reversal sequence for FtsK. In Chapter 2, I use a continuous ensemble assay for dsDNA translocation to show that FtsK initiates rapidly at KOPS, with loading dependent on FtsKgamma. Translocation requires moderately cooperative ATP binding, while ATP hydrolysis has a more relaxed cooperativity. I have determined the ATP coupling efficiency of translocation to be ~1.6 bp/ATP, in line with theoretical estimates. Though FtsK probably strips most proteins from DNA, I show in Chapter 3 that FtsK stops translocating when it encounters XerCD bound to dif. The interaction is most likely a specific down-regulation, but surprisingly does not depend on FtsKgamma or on the catalytic or synaptic activity of XerCD. In Chapter 4, I show some preliminary structural data of FtsKC bound to dsDNA, with the aim of determining the first high resolution structure of a ring dsDNA translocase bound to nucleic acid.

Published

2010

26. Researchers at University of Maryland Release New Data on Life Science (Anthrax Toxin: Model System for Studying Protein Translocation).

Abstract

Researchers at the University of Maryland have released new data on the use of anthrax toxin as a model system for studying protein translocation. The research focuses on the unfolding and translocation of proteins through nanomachines called translocase channels. These channels utilize peptide-clamp active sites to catalyze unfolding and translocation, and are powered by the endosomal proton gradient. The research compares and contrasts anthrax toxin with other translocase channels. This information may be useful for those studying life science and protein translocation. [Extracted from the article]

Published

2024

27. Enhanced delivery of protein therapeutics with a diphtheria toxin-like platform that evades pre-existing neutralizing immunity.

Abstract

According to a preprint abstract, researchers have discovered a new delivery platform for therapeutic peptides and proteins called Chelona Toxin (CT). CT is a distant diphtheria toxin homolog that is structurally and functionally similar to diphtheria toxin (DT), but it is not recognized by pre-existing anti-DT antibodies in human sera. The researchers found that CT is superior to DT at delivering therapeutic protein cargo into target cells. This discovery could potentially lead to the development of safer and more effective immunotoxins and intracellular protein delivery platforms for cancer therapy. However, it is important to note that this preprint has not yet been peer-reviewed. [Extracted from the article]

Published

2024

28. Patent Issued for Use of PPAR-delta agonists in the treatment of disease (USPTO 11931365).

Subjects

THERAPEUTICS, CARNITINE palmitoyltransferase, PATENTS, GLYCOGEN storage disease, MITOCHONDRIAL DNA

Abstract

Reneo Pharmaceuticals Inc. has been issued a patent for the use of PPAR-delta agonists in the treatment of various diseases and disorders. The patent describes a method for treating conditions such as muscle atrophy, mitochondrial myopathy, fatty acid oxidation disorders, kidney disease, glycogen storage disease, and more. The inventors claim that the administration of a specific compound, sodium (E)-2-(4-((3-(4-fluorophenyl)-3-(4-(3-morpholinoprop-1-yn-1-yl)phenyl)allyl)oxy)-2-methylphenoxy)acetate, can improve exercise tolerance, muscle histology, cognition, overall well-being, and reduce pain and fatigue in patients with these conditions. The patent provides detailed information on the dosage and administration of the compound. [Extracted from the article]

Published

2024

29. Data from Clinical Hospital Advance Knowledge in Fatty Liver Disease (Essential Lipid Autacoids Rewire Mitochondrial Energy Efficiency In Metabolic Dysfunction-associated Fatty Liver Disease).

Subjects

FATTY liver, ENERGY consumption, MITOCHONDRIA, DIGESTIVE system diseases, LIPIDS, OMEGA-6 fatty acids

Abstract

A study conducted in Barcelona, Spain, explored the impact of changes in essential fatty acid-derived lipid autacoids on hepatocyte mitochondrial bioenergetics and metabolic efficiency in metabolic dysfunction-associated fatty liver disease. The study used transgenic mice with the fat-1 gene, which allows for the replacement of omega-6-polyunsaturated fatty acids with omega-3 polyunsaturated fatty acids. The results showed that mice with the fat-1 gene had improved mitochondrial function, increased expression of oxidative phosphorylation complexes, and enhanced energy substrate utilization. The study highlights the importance of a lipid membrane composition rich in docosahexaenoic acid and its lipid autacoid derivatives for optimal hepatic mitochondrial and metabolic efficiency. [Extracted from the article]

Published

2024

30. Analysis of mitochondrial protein translocation by disulfide bond formation and cysteine specific crosslinking.

Author

Fielden LF, Busch JD, Lindau C, Qiu J, and Wiedemann N

Subjects

Mitochondria metabolism, Mitochondria chemistry, Humans, Mitochondrial Precursor Protein Import Complex Proteins, Cysteine chemistry, Cysteine metabolism, Disulfides chemistry, Disulfides metabolism, Protein Transport, Mitochondrial Proteins metabolism, Mitochondrial Proteins chemistry, Mitochondrial Proteins genetics, Cross-Linking Reagents chemistry

Abstract

Protein translocation is a highly dynamic process and, in addition, mitochondrial protein import is especially complicated as the majority of nuclear encoded precursor proteins must engage with multiple translocases before they are assembled in the correct mitochondrial subcompartment. In this chapter, we describe assays for engineered disulfide bond formation and cysteine specific crosslinking to analyze the rearrangement of translocase subunits or to probe protein-protein interactions between precursor proteins and translocase subunits. Such assays were used to characterize the translocase of the outer membrane, the presequence translocase of the inner membrane and the sorting and assembly machinery for the biogenesis of β-Barrel proteins. Moreover, these approaches were also employed to determine the translocation path of precursor proteins (identification of import receptors and specific domains required for translocation) as well as the analysis, location and translocase subunit dependence for the formation of β-Barrel proteins. Here we describe how engineered disulfide bond formation and cysteine specific crosslinking assays are planned and performed and discuss important aspects for its application to study mitochondrial protein translocation., (Copyright © 2024. Published by Elsevier Inc.)

Published

2024

31. Monitoring the in vitro import and assembly of mitochondrial precursor proteins into mammalian mitochondria.

Author

Crameri JJ and Stojanovski D

Subjects

Animals, Humans, Protein Precursors metabolism, Mitochondrial Membranes metabolism, Protein Transport, Mitochondria metabolism, Mitochondrial Proteins metabolism

Abstract

Mitochondrial protein import is a complex process governing the delivery of the organelle's proteome. This process, in turn, is essential for maintaining mitochondrial function and cellular homeostasis. Initiated by protein synthesis in the cytoplasm, precursor proteins destined for the mitochondria possess targeting signals that guide them to the mitochondrial surface. At mitochondria, the translocation of proteins across the mitochondrial membranes involves an intricate interplay between translocases, chaperones, and receptors. The mitochondrial import assay offers researchers the opportunity to recapitulate the process of protein import in vitro. The assay has served as an indispensable tool in helping decipher the intricacies of protein translocation into mitochondria, first in fungal models, and subsequently in higher eukaryotic models. In this chapter, we will describe how protein import can be assayed using mammalian mitochondria and provide insight into the types of questions that can be addressed in mammalian mitochondrial biology using this experimental approach., (Copyright © 2024. Published by Elsevier Inc.)

Published

2024

32. The Principles of Protein Targeting and Transport Across Cell Membranes.

Author

Chen, Yuanyuan, Shanmugam, Sri Karthika, and Dalbey, Ross E.

Subjects

*CARRIER proteins, *CELL membranes, *MEMBRANE proteins, *TIME measurements, *PROTEINS

Abstract

The past several decades have witnessed tremendous growth in the protein targeting, transport and translocation field. Major advances were made during this time period. Now the molecular details of the targeting factors, receptors and the membrane channels that were envisioned in Blobel's Signal Hypothesis in the 1970s have been revealed by powerful structural methods. It is evident that there is a myriad of cytosolic and membrane associated systems that accurately sort and target newly synthesized proteins to their correct membrane translocases for membrane insertion or protein translocation. Here we will describe the common principles for protein transport in prokaryotes and eukaryotes. [ABSTRACT FROM AUTHOR]

Published

2019

33. Calcium‐regulated mitochondrial ATP‐Mg/Pi carriers evolved from a fusion of an EF‐hand regulatory domain with a mitochondrial ADP/ATP carrier‐like domain.

Author

Harborne, Steven P. D. and Kunji, Edmund R. S.

Subjects

*ADENINE nucleotides, *CALMODULIN, *ADENOSINE triphosphate, *MITOCHONDRIA, *ADENOSINE diphosphate

Abstract

The mitochondrial ATP‐Mg/Pi carrier is responsible for the calcium‐dependent regulation of adenosine nucleotide concentrations in the mitochondrial matrix, which allows mitochondria to respond to changing energy requirements of the cell. The carrier is expressed in mitochondria of fungi, plants and animals and belongs to the family of mitochondrial carriers. The carrier is unusual as it consists of three separate domains: (i) an N‐terminal regulatory domain with four calcium‐binding EF‐hands similar to calmodulin, (ii) a loop domain containing an amphipathic α‐helix and (iii) a mitochondrial carrier domain related to the mitochondrial ADP/ATP carrier. This striking example of three domains coming together from different origins to provide new functions represents an interesting quirk of evolution. In this review, we outline how the carrier was identified and how its physiological role was established with a focus on human isoforms. We exploit the sequence and structural information of the domains to explore the similarities and differences to their closest counterparts; mitochondrial ADP/ATP carriers and proteins with four EF‐hands. We discuss how their combined function has led to a mechanism for calcium‐regulated transport of adenosine nucleotides. Finally, we compare the ATP‐Mg/Pi carrier with the mitochondrial aspartate/glutamate carrier, the only other mitochondrial carrier regulated by calcium, and we will argue that they have arisen by convergent rather than divergent evolution. © 2018 The Authors. IUBMB Life published by Wiley Periodicals, Inc. on behalf of International Union of Biochemistry and Molecular Biology, 70(12):1222–1232, 2018 [ABSTRACT FROM AUTHOR]

Published

2018

34. Researcher at Pirogov Russian National Research Medical University Describes Research in Ophthalmic Antiinflammatory Agents (Possible Participation of Adenine Nucleotide Translocase ANT1 in the Cytotoxic Action of Progestins, Glucocorticoids,...).

Abstract

A recent study conducted at Pirogov Russian National Research Medical University in Moscow explored the cytostatic effects of progestins, glucocorticoids, and diclofenac on tumor cells. The researchers found that different cell lines exhibited varying sensitivities to these drugs. Progestin gestobutanoyl was the most cytotoxic, while glucocorticoids and diclofenac were less cytotoxic. The study also examined the expression of adenylate nucleotide translocase ANT1 as a possible participant in the cytotoxic action of these drugs. The modulation of ANT1 expression could provide new insights into the cytotoxic and cytoprotective effects of hormones and anti-inflammatory drugs. [Extracted from the article]

Published

2024

35. Southeast University Researcher Provides New Insights into Liposomes [Astragalus polysaccharide liposome nanoparticles mediate fatty acid translocase (FAT)/CD36 to improve fatty acid metabolism and regulate glucocorticoid receptor levels in...].

Abstract

A study conducted by researchers at Southeast University in China has found that Astragalus polysaccharide (APS) combined with liposome nanoparticles (APS-nano) can improve fatty acid metabolism and regulate glucocorticoid receptor levels in diabetic cardiomyopathy (DCM). The study involved 50 rats and compared the effects of APS-nano with other groups. The results showed that APS-nano had the highest level of insulin and the lowest blood sugar levels among all groups. It also decreased the levels of total cholesterol, triglyceride, and free fatty acid compared to the control and model groups. The study concluded that APS-nano can regulate FAT/CD36 expression and improve fatty acid metabolism, thereby lowering myocardial tissue metabolism and inhibiting glucocorticoid receptor levels. [Extracted from the article]

Published

2023

36. Immortalised murine R349P desmin knock-in myotubes exhibit a reduced proton leak and decreased ADP/ATP translocase levels in purified mitochondria.

Abstract

A recent preprint abstract discusses the findings of a study on the effects of a specific gene mutation on mitochondrial function in muscle tissue. The researchers used skeletal muscle myoblasts from mice with the gene mutation to create an immortalized cellular disease model. They found that the myotubes derived from these cells showed disruptions in the desmin cytoskeleton and myofibrillar irregularities. Additionally, the mitochondria from these cells exhibited a reduced proton leak and decreased levels of ADP/ATP translocases, suggesting a potential early step in the development of secondary mitochondriopathy. It is important to note that this preprint has not yet undergone peer review. [Extracted from the article]

Published

2023

37. Synthetic Sansanmycin Analogues as Potent Mycobacterium tuberculosis Translocase I Inhibitors

Author

Elinor Hortle, David I. Roper, Warwick J. Britton, Richard J. Payne, Gregory M. Cook, Wendy Tran, Paige M. E. Hawkins, Alexander Stoye, Christopher G. Dowson, Rebecca E Audette, Thomas Balle, Jessica L. Ochoa, Gayathri Nagalingam, Daniel J Ford, Ali Saad Kusay, Venugopal Pujari, Roger G. Linington, Chen-Yi Cheung, Dean C. Crick, Eric J. Rubin, Stefan H. Oehlers, and Susan A. Charman

Subjects

Natural product, Tuberculosis, biology, medicine.drug_class, Isoniazid, bacterial infections and mycoses, Antimycobacterial, biology.organism_classification, medicine.disease, In vitro, Mycobacterium tuberculosis, chemistry.chemical_compound, chemistry, Biochemistry, In vivo, Drug Discovery, biology.protein, medicine, Molecular Medicine, Translocase, medicine.drug

Abstract

Herein, we report the design and synthesis of inhibitors of Mycobacterium tuberculosis (Mtb) phospho-MurNAc-pentapeptide translocase I (MurX), the first membrane-associated step of peptidoglycan synthesis, leveraging the privileged structure of the sansanmycin family of uridylpeptide natural products. A number of analogues bearing hydrophobic amide modifications to the pseudo-peptidic end of the natural product scaffold were generated that exhibited nanomolar inhibitory activity against Mtb MurX and potent activity against Mtb in vitro. We show that a lead analogue bearing an appended neopentylamide moiety possesses rapid antimycobacterial effects with a profile similar to the frontline tuberculosis drug isoniazid. This molecule was also capable of inhibiting Mtb growth in macrophages where mycobacteria reside in vivo and reduced mycobacterial burden in an in vivo zebrafish model of tuberculosis.

Published

2021

38. Helical inchworming: a novel translocation mechanism for a ring ATPase

Author

Alexander B. Tong and Carlos Bustamante

Subjects

Ring atpase, biology, Chemistry, ATPase, Biophysics, Membrane biology, Optical tweezers, Chromosomal translocation, Ring (chemistry), biology.organism_classification, Bacteriophage, Structural Biology, Translocase, Commentary, Molecular motor, biology.protein, Cryo-electron microscopy, Molecular Biology, Function (biology)

Abstract

Ring ATPases perform a variety of tasks in the cell. Their function involves complex communication and coordination among the often identical subunits. Translocases in this group are of particular interest as they involve both chemical and mechanical actions in their operation. We study the DNA packaging motor of bacteriophage φ29, and using single-molecule optical tweezers and single-particle cryo-electron microscopy, have discovered a novel translocation mechanism for a molecular motor.

Published

2021

39. Engineering a Supersecreting Strain of Escherichia coli by Directed Coevolution of the Multiprotein Tat Translocation Machinery

Author

May N. Taw, Dujduan Waraho-Zhmayev, Matthew P. DeLisa, Mark A. Rocco, Daniel Kim, and Mingji Li

Subjects

biology, Chemistry, Mutant, Biomedical Engineering, Heterologous, General Medicine, Periplasmic space, medicine.disease_cause, Directed evolution, Biochemistry, Genetics and Molecular Biology (miscellaneous), Cell biology, Twin-arginine translocation pathway, biology.protein, Protein biosynthesis, medicine, Translocase, Escherichia coli

Abstract

Escherichia coli remains one of the preferred hosts for biotechnological protein production due to its robust growth in culture and ease of genetic manipulation. It is often desirable to export recombinant proteins into the periplasmic space for reasons related to proper disulfide bond formation, prevention of aggregation and proteolytic degradation, and ease of purification. One such system for expressing heterologous secreted proteins is the twin-arginine translocation (Tat) pathway, which has the unique advantage of delivering correctly folded proteins into the periplasm. However, transit times for proteins through the Tat translocase, comprised of the TatABC proteins, are much longer than for passage through the SecYEG pore, the translocase associated with the more widely utilized Sec pathway. To date, a high protein flux through the Tat pathway has yet to be demonstrated. To address this shortcoming, we employed a directed coevolution strategy to isolate mutant Tat translocases for their ability to deliver higher quantities of heterologous proteins into the periplasm. Three supersecreting translocases were selected that each exported a panel of recombinant proteins at levels that were significantly greater than those observed for wild-type TatABC or SecYEG translocases. Interestingly, all three of the evolved Tat translocases exhibited quality control suppression, suggesting that increased translocation flux was gained by relaxation of substrate proofreading. Overall, our discovery of more efficient translocase variants paves the way for the use of the Tat system as a powerful complement to the Sec pathway for secreted production of both commodity and high value-added proteins.

Published

2021

40. How Does a Helicase Unwind DNA? Insights from RecBCD Helicase.

Author

Lohman, Timothy M. and Fazio, Nicole T.

Subjects

*DNA helicases, *MOLECULAR motor proteins, *ESCHERICHIA coli, *EXONUCLEASES, *NUCLEOTIDE sequence, *SINGLE-stranded DNA

Abstract

DNA helicases are a class of molecular motors that catalyze processive unwinding of double stranded DNA. In spite of much study, we know relatively little about the mechanisms by which these enzymes carry out the function for which they are named. Most current views are based on inferences from crystal structures. A prominent view is that the canonical ATPase motor exerts a force on the ssDNA resulting in “pulling” the duplex across a “pin” or “wedge” in the enzyme leading to a mechanical separation of the two DNA strands. In such models, DNA base pair separation is tightly coupled to ssDNA translocation of the motors. However, recent studies of the Escherichia coli RecBCD helicase suggest an alternative model in which DNA base pair melting and ssDNA translocation occur separately. In this view, the enzyme‐DNA binding free energy is used to melt multiple DNA base pairs in an ATP‐independent manner, followed by ATP‐dependent translocation of the canonical motors along the newly formed ssDNA tracks. Repetition of these two steps results in processive DNA unwinding. We summarize recent evidence suggesting this mechanism for RecBCD helicase action. [ABSTRACT FROM AUTHOR]

Published

2018

41. Coordinated motion of molecular motors on DNA chains with branch topology

Author

Bin Chen and Di Lu

Subjects

Physics, biology, Mechanical Engineering, Computational Mechanics, Topology, chemistry.chemical_compound, Molecular level, Chain (algebraic topology), chemistry, Self-healing hydrogels, Molecular motor, biology.protein, Translocase, Topology (chemistry), DNA

Abstract

Toward understanding the macroscopic mechanical behaviors of responsive deoxyribonucleic acid (DNA) hydrogels integrated with DNA motors, here we construct the state map for the translocation process of a single C-terminal translocase domain (FtsKC) on a single DNA chain at the molecular level and then investigate the movement of single or multiple FtsKC motors on DNA chains with varied branch topology. Our studies indicate that multiple FtsKC motors can have coordinated motion, which is mainly due to the force responsive behavior of individual FtsKC motor. We further suggest the potential application of motors of FtsKC, together with DNA chains of specific branch topology, to serve as strain sensors in hydrogels.

Published

2021

42. Tomatidine provides mitophagy‐independent neuroprotection after ischemic injury

Author

Anil Ahsan, Li-na Zhang, Zikai Feng, Xiangnan Zhang, Yu-ting Wang, Yue Li, and Xiao-cui Lyu

Subjects

autophagy, Cell Survival, QH301-705.5, Ischemia, Mitochondrion, Pharmacology, Neuroprotection, cerebral ischemia, General Biochemistry, Genetics and Molecular Biology, Brain Ischemia, Neuroblastoma cell, Mice, Tomatine, Cell Line, Tumor, Mitophagy, medicine, Animals, Humans, Translocase, Biology (General), Research Articles, Neurons, biology, business.industry, Autophagy, Ischemic injury, medicine.disease, Mitochondria, Oxygen, Glucose, Neuroprotective Agents, mitophagy, biology.protein, business, tomatidine, Research Article

Abstract

Cerebral ischemia is one of the leading causes of human mortality and disability worldwide. The treatment of cerebral ischemia is refractory due to its short therapeutic window and lack of effective clinical drugs. Mitophagy, the autophagic elimination of damaged mitochondria, attenuates neuronal injury in cerebral ischemia, indicating the potential of mitophagy inducers as therapies for cerebral ischemia. We previously determined that, by enhancing autophagy flux, the steroidal alkaloid tomatidine can function as a neuroprotective agent against ischemic injury. However, its effects on mitophagy remain unknown. For this purpose, neuroblastoma cell lines Neuro‐2a and SH‐SY5Y were subjected to ischemic injury induced by oxygen–glucose deprivation/reperfusion (OGD/R) and then treated with tomatidine. OGD/R induced a general decrease of cellular contents, and this study revealed that tomatidine had no impact on mitophagy. In addition, tomatidine did not affect mitochondrial contents, including translocase of outer mitochondrial membrane 20 and voltage‐dependent anion channel 1, in either OGD/R‐treated or intact SH‐SY5H cells. Our results indicate that tomatidine exhibits its neuroprotective effects by enhancing autophagy, but in a potentially mitophagy‐independent manner, and provide insights for further investigation into its mechanism(s) and potential therapeutic use against cerebral ischemia., The steroidal alkaloid, tomatidine, has been shown to treat cerebral ischemia by enhancing autophagy, but its effect on mitophagy is still unknown. Our work indicates that the neuroprotective role of tomatidine is independent of mitophagy. Further research should be performed to determine how autophagy contributes to the neuroprotective effects of tomatidine in ischemic neurons.

Published

2021

43. The lane-switch mechanism for nucleosome repositioning by DNA translocase

Author

Fritz Nagae, Giovanni B. Brandani, Tsuyoshi Terakawa, and Shoji Takada

Subjects

biology, AcademicSubjects/SCI00010, DNA Helicases, Helicase, Computational Biology, Eukaryotic DNA replication, DNA-Directed RNA Polymerases, Molecular Dynamics Simulation, Chromatin Assembly and Disassembly, Cell biology, Nucleosomes, Histones, chemistry.chemical_compound, Histone, Exodeoxyribonucleases, chemistry, Transcription (biology), Genetics, biology.protein, Nucleosome, Translocase, Humans, DNA, Polymerase

Abstract

Translocases such as DNA/RNA polymerases, replicative helicases, and exonucleases are involved in eukaryotic DNA transcription, replication, and repair. Since eukaryotic genomic DNA wraps around histone octamers and forms nucleosomes, translocases inevitably encounter nucleosomes. A previous study has shown that a nucleosome repositions downstream when a translocase collides with the nucleosome. However, the molecular mechanism of the downstream repositioning remains unclear. In this study, we identified the lane-switch mechanism for downstream repositioning with molecular dynamics simulations and validated it with restriction enzyme digestion assays and deep sequencing assays. In this mechanism, after a translocase unwraps nucleosomal DNA up to the site proximal to the dyad, the remaining wrapped DNA switches its binding lane to that vacated by the unwrapping, and the downstream DNA rewraps, completing downstream repositioning. This mechanism may have broad implications for transcription through nucleosomes, histone recycling, and nucleosome remodeling.

Published

2021

44. Identification of Arginine Finger as the Starter of the Biomimetic Motor in Driving Double-Stranded DNA

Author

Chenxi Liang and Peixuan Guo

Subjects

Arginine, Protein subunit, ATPase, General Physics and Astronomy, phi29 DNA packaging, Random hexamer, Article, viral assembly, chemistry.chemical_compound, Adenosine Triphosphate, Biomimetics, Transcription (biology), DNA Packaging, Translocase, General Materials Science, DNA-packaging motor, Adenosine Triphosphatases, sequential action, biology, Chemistry, Virus Assembly, Walker motifs, General Engineering, Cell biology, revolving motor, DNA, Viral, biology.protein, asymmetrical hexameric ATPase, inchworm, DNA

Abstract

Nanomotors in nanotechnology may be as important as cars in daily life. Biomotors are nanoscale machines ubiquitous in living systems to carry out ATP-driven activities such as walking, breathing, blinking, mitosis, replication, transcription, and trafficking. The sequential action in an asymmetrical hexamer by a revolving mechanism has been confirmed in dsDNA packaging motors of phi29, herpesviruses, bacterial dsDNA translocase FtsK, and Streptomyces TraB for conjugative dsDNA transfer. These elaborate, delicate, and exquisite ring structures have inspired scientists to design biomimetics in nanotechnology. Many multisubunit ATPase rings generate force via sequential action of multiple modules, such as the Walker A, Walker B, P-loop, arginine finger, sensors, and lid. The chemical to mechanical energy conversion usually takes place in sequential order. It is commonly believed that ATP binding triggers such conversion, but how the multimodule motor starts the sequential process has not been explicitly investigated. Identification of the starter is of great significance for biomimetic motor fabrication. Here, we report that the arginine finger is the starter of the motor. Only one amino acid residue change in the arginine finger led to the impediment and elimination of all following steps. Without the arginine finger, the motor failed to assemble, bind ATP, recruit DNA, or hydrolyze ATP and was eventually unable to package DNA. However, the loss of ATPase activity due to an inactive arginine finger can be rescued by an arginine finger from the adjacent subunit of Walker A mutant through trans-complementation. Taken together, we demonstrate that the formation of dimers triggered by the arginine finger initiates the motor action rather than the general belief of initiation by ATP binding.

Published

2021

45. Ribosome as a Translocase and Helicase

Author

Dmitri N. Ermolenko and Chen Bao

Subjects

Models, Molecular, Base pair, power stroke, translocation, Review, Biochemistry, Ribosome, Peptide Elongation Factor 2, RNA, Transfer, Transferases, Fluorescence Resonance Energy Transfer, Protein biosynthesis, Translocase, RNA, Messenger, Messenger RNA, biology, Chemistry, Cryoelectron Microscopy, Eukaryota, Helicase, Biological Transport, General Medicine, Ribosomal RNA, Peptide Elongation Factor G, Cell biology, Elongation factor, helicase, ribosome, Protein Biosynthesis, biology.protein, Brownian ratchet, Ribosomes, RNA Helicases

Abstract

During protein synthesis, ribosome moves along mRNA to decode one codon after the other. Ribosome translocation is induced by a universally conserved protein, elongation factor G (EF-G) in bacteria and elongation factor 2 (EF-2) in eukaryotes. EF-G-induced translocation results in unwinding of the intramolecular secondary structures of mRNA by three base pairs at a time that renders the translating ribosome a processive helicase. Professor Alexander Sergeevich Spirin has made numerous seminal contributions to understanding the molecular mechanism of translocation. Here, we review Spirin's insights into the ribosomal translocation and recent advances in the field that stemmed from Spirin's pioneering work. We also discuss key remaining challenges in studies of translocase and helicase activities of the ribosome.

Published

2021

46. Outer and inner mitochondrial membrane proteins <scp>TOMM40</scp> and <scp>TIMM50</scp> are intensively concentrated and localized at Purkinje and pyramidal neurons in the New Zealand white rabbit brain

Author

Elsayed Metwally, Ahmed A. H. Abdellatif, and Sameh M. Farouk

Subjects

0301 basic medicine, Cerebellum, Histology, Mitochondrion, 03 medical and health sciences, 0302 clinical medicine, Mitochondrial Precursor Protein Import Complex Proteins, medicine, Animals, Translocase, Cytochrome c oxidase, Inner mitochondrial membrane, Ecology, Evolution, Behavior and Systematics, Cellular localization, biology, Chemistry, Cerebrum, Pyramidal Cells, Brain, Mitochondria, Cell biology, 030104 developmental biology, medicine.anatomical_structure, nervous system, Cytoplasm, Mitochondrial Membranes, biology.protein, Rabbits, Anatomy, Carrier Proteins, 030217 neurology & neurosurgery, Biotechnology

Abstract

Mitochondria are involved in a variety of developmental processes and neurodegenerative diseases. The translocase complexes of the outer and inner mitochondrial membranes (TOM and TIM) are protein complexes involved in transporting protein precursors across mitochondrial membranes. Although rabbits are important animal models for neurodegenerative diseases, the expression of TOM and TIM complexes has yet to be examined in the rabbit brain. In the present study, we quantitatively evaluated the protein expression of the translocase of outer mitochondrial membrane 40 (TOMM40) and inner mitochondrial membrane 50 (TIMM50) complexes, two of the TOM/TIM complexes, in the cerebral, cerebellar, and hippocampal cortices of the New Zealand white rabbit brain, using immunohistochemistry. Sections from brain specimens were initially stained for cytochrome c oxidase (COX), a well-known mitochondrial marker, which was found to be homogeneously expressed in the cerebrum, but localized to the Purkinje and pyramidal neurons of the cerebellum and hippocampus, respectively. TOMM40 and TIMM50 proteins consistently revealed a similar expression pattern, although at different ratios. In the cerebrum, TOMM40 and TIMM50 immunoreactions were homogeneously distributed within the cytoplasm of various neurons. Meanwhile, Purkinje cells in the cerebellum and pyramidal neurons in the hippocampus displayed higher intensities in their cytoplasm. The specific cellular localization of TOMM40 and TIMM50 proteins in various regions of the rabbit brain suggests a distinct function of each protein in these regions. Further analysis will be required to evaluate the molecular functions of these proteins.

Published

2021

47. Long DNA constructs to study helicases and nucleic acid translocases using optical tweezers

Author

European Research Council, Ministerio de Economía y Competitividad (España), Comunidad de Madrid, Wellcome Trust, University of Bristol, Aicart-Ramos, Clara, Hormeño, Silvia, Wilkinson, Oliver J., Dillingham, Mark Simon, Moreno-Herrero, Fernando, European Research Council, Ministerio de Economía y Competitividad (España), Comunidad de Madrid, Wellcome Trust, University of Bristol, Aicart-Ramos, Clara, Hormeño, Silvia, Wilkinson, Oliver J., Dillingham, Mark Simon, and Moreno-Herrero, Fernando

Abstract

Single molecule biophysics experiments for the study of DNA-protein interactions usually require production of a homogeneous population of long DNA molecules with controlled sequence content and/or internal tertiary structures. Traditionally, Lambda phage DNA has been used for this purpose, but it is difficult to customize. In this article, we provide a detailed and simple protocol for cloning large (~ 25 kbp) plasmids with bespoke sequence content, which can be used to generate custom DNA constructs for a range of single-molecule experiments. In particular, we focus on a procedure for making long single-stranded DNA (ssDNA) molecules, ssDNA-dsDNA hybrids and long DNA constructs with flaps, which are especially relevant for studying the activity of DNA helicases and translocases. Additionally, we describe how the modification of the free ends of such substrates can facilitate their binding to functionalized surfaces allowing immobilization and imaging using dual optical tweezers and confocal microscopy. Finally, we provide examples of how these DNA constructs have been applied to study the activity of human DNA helicase B (HELB). The techniques described herein are simple, versatile, adaptable, and accessible to any laboratory with access to standard molecular biology methods.

Published

2022

48. All motors have to decide is what to do with the DNA that is given them

Author

Briggs Koan and Fischer Christopher J.

Subjects

atpase, molecular motor, translocase, Biology (General), QH301-705.5

Abstract

DNA translocases are a diverse group of molecular motors responsible for a wide variety of cellular functions. The goal of this review is to identify common aspects in the mechanisms for how these enzymes couple the binding and hydrolysis of ATP to their movement along DNA. Not surprisingly, the shared structural components contained within the catalytic domains of several of these motors appear to give rise to common aspects of DNA translocation. Perhaps more interesting, however, are the differences between the families of translocases and the potential associated implications both for the functions of the members of these families and for the evolution of these families. However, as there are few translocases for which complete characterizations of the mechanisms of DNA binding, DNA translocation, and DNA-stimulated ATPase have been completed, it is difficult to form many inferences. We therefore hope that this review motivates the necessary further experimentation required for broader comparisons and conclusions.

Published

2014

49. Structural insights into assembly of human mitochondrial translocase TOM complex

Author

Ling Yan, Liangbo Qi, Zeyuan Guan, Ping Yin, Zhou Gong, Qiang Wang, Chuangye Yan, and Sixing Hong

Subjects

Protein translocation, biology, QH573-671, Chemistry, TIM/TOM complex, Cell Biology, Computational biology, Biochemistry, Cryoelectron microscopy, Correspondence, Genetics, biology.protein, Translocase, Cytology, Molecular Biology

Published

2021

50. Oligomeric quaternary structure of Escherichia coli and Mycobacterium smegmatis Lhr helicases is nucleated by a novel C-terminal domain composed of five winged-helix modules

Author

Dinshaw J. Patel, Garrett M Warren, Juncheng Wang, and Stewart Shuman

Subjects

DNA, Bacterial, AcademicSubjects/SCI00010, Stereochemistry, Escherichia coli Proteins, Mycobacterium smegmatis, Protein domain, DNA Helicases, Helicase, Protomer, Genome Integrity, Repair and Replication, Biology, biology.organism_classification, environment and public health, Protein tertiary structure, RNA, Bacterial, chemistry.chemical_compound, Protein Domains, chemistry, Escherichia coli, Genetics, biology.protein, Translocase, Protein quaternary structure, DNA

Abstract

Mycobacterium smegmatis Lhr (MsmLhr; 1507-aa) is the founder of a novel clade of bacterial helicases. MsmLhr consists of an N-terminal helicase domain (aa 1–856) with a distinctive tertiary structure (Lhr-Core) and a C-terminal domain (Lhr-CTD) of unknown structure. Here, we report that Escherichia coli Lhr (EcoLhr; 1538-aa) is an ATPase, translocase and ATP-dependent helicase. Like MsmLhr, EcoLhr translocates 3′ to 5′ on ssDNA and unwinds secondary structures en route, with RNA:DNA hybrid being preferred versus DNA:DNA duplex. The ATPase and translocase activities of EcoLhr inhere to its 877-aa Core domain. Full-length EcoLhr and MsmLhr have homo-oligomeric quaternary structures in solution, whereas their respective Core domains are monomers. The MsmLhr CTD per se is a homo-oligomer in solution. We employed cryo-EM to solve the structure of the CTD of full-length MsmLhr. The CTD protomer is composed of a series of five winged-helix (WH) modules and a β-barrel module. The CTD adopts a unique homo-tetrameric quaternary structure. A Lhr-CTD subdomain, comprising three tandem WH modules and the β-barrel, is structurally homologous to AlkZ, a bacterial DNA glycosylase that recognizes and excises inter-strand DNA crosslinks. This homology is noteworthy given that Lhr is induced in mycobacteria exposed to the inter-strand crosslinker mitomycin C.

Published

2021