Your search keyword '"Ankyrin repeat"' showing total 2,649 results

1. A designed ankyrin-repeat protein that targets Parkinsons disease-associated LRRK2.

Author

Dederer, Verena, Sanz Murillo, Marta, Karasmanis, Eva, Hatch, Kathryn, Chatterjee, Deep, Preuss, Franziska, Abdul Azeez, Kamal, Nguyen, Landon, Galicia, Christian, Dreier, Birgit, Plückthun, Andreas, Versees, Wim, Mathea, Sebastian, Leschziner, Andres, Reck-Peterson, Samara, and Knapp, Stefan

Subjects

DARPin, LRRK2, Parkinson’s disease, Rab8a, WD40, cryo-electron microscopy, kinase, kinase inhibitor, microtubule, Leucine-Rich Repeat Serine-Threonine Protein Kinase-2, Humans, Ankyrin Repeat, Parkinson Disease, HEK293 Cells, rab GTP-Binding Proteins, Phosphorylation, Cryoelectron Microscopy, Protein Binding

Abstract

Leucine rich repeat kinase 2 (LRRK2) is a large multidomain protein containing two catalytic domains, a kinase and a GTPase, as well as protein interactions domains, including a WD40 domain. The association of increased LRRK2 kinase activity with both the familial and sporadic forms of Parkinsons disease has led to an intense interest in determining its cellular function. However, small molecule probes that can bind to LRRK2 and report on or affect its cellular activity are needed. Here, we report the identification and characterization of the first high-affinity LRRK2-binding designed ankyrin-repeat protein (DARPin), named E11. Using cryo-EM, we show that DARPin E11 binds to the LRRK2 WD40 domain. LRRK2 bound to DARPin E11 showed improved behavior on cryo-EM grids, resulting in higher resolution LRRK2 structures. DARPin E11 did not affect the catalytic activity of a truncated form of LRRK2 in vitro but decreased the phosphorylation of Rab8A, a LRRK2 substrate, in cells. We also found that DARPin E11 disrupts the formation of microtubule-associated LRRK2 filaments in cells, which are known to require WD40-based dimerization. Thus, DARPin E11 is a new tool to explore the function and dysfunction of LRRK2 and guide the development of LRRK2 kinase inhibitors that target the WD40 domain instead of the kinase.

Published

2024

2. X-ray crystal structure of a designed rigidified imaging scaffold in the ligand-free conformation.

Author

Agdanowski, Matthew, Castells-Graells, Roger, Sawaya, Michael, Cascio, Duilio, Yeates, Todd, and Arbing, Mark

Subjects

DARPins, imaging scaffolds, protein cages, protein design, Crystallography, X-Ray, Models, Molecular, Ankyrin Repeat, Cryoelectron Microscopy, Ligands, Protein Conformation, Protein Binding, Gene Expression

Abstract

Imaging scaffolds composed of designed protein cages fused to designed ankyrin repeat proteins (DARPins) have enabled the structure determination of small proteins by cryogenic electron microscopy (cryo-EM). One particularly well characterized scaffold type is a symmetric tetrahedral assembly composed of 24 subunits, 12 A and 12 B, which has three cargo-binding DARPins positioned on each vertex. Here, the X-ray crystal structure of a representative tetrahedral scaffold in the apo state is reported at 3.8 Å resolution. The X-ray crystal structure complements recent cryo-EM findings on a closely related scaffold, while also suggesting potential utility for crystallographic investigations. As observed in this crystal structure, one of the three DARPins, which serve as modular adaptors for binding diverse `cargo proteins, present on each of the vertices is oriented towards a large solvent channel. The crystal lattice is unusually porous, suggesting that it may be possible to soak crystals of the scaffold with small (≤30 kDa) protein cargo ligands and subsequently determine cage-cargo structures via X-ray crystallography. The results suggest the possibility that cryo-EM scaffolds may be repurposed for structure determination by X-ray crystallography, thus extending the utility of electron-microscopy scaffold designs for alternative structural biology applications.

Published

2024

3. Exploring Genetic Factors Involved in the Risk of Bruxism in Male Construction Workers

Author

Michelle Nascimento Meger, Samantha Schaffer Pugsley Baratto, Bianca Cavalcante- Leao, Maria Eduarda Nunis Locks, Camila Paiva Perin, Gisele Maria Correr, Natanael Henrique Mattos, Christian Kirschneck, Erika Calvano Küchler, and Flares Baratto-Filho

Subjects

Bruxism, ankyrin repeat, men, dopamine, Dentistry, RK1-715

Abstract

ABSTRACTObjective The bruxism has a multifactorial etiology, in which molecular factors and genes play an important role. Dopaminergic pathways are pathways involved in functions such as motor control, reward, motivation, arousal and cognition. Genetic polymorphisms in the genes encoding Dopamine Receptor D2 (DRD2) and Ankyrin Repeat and Kinase Domain Containing 1 (ANKK1) have been reported in the literature associated with sleep disorders, migraine, personality, acute and chronic pain.Methods The present study aimed to assess whether genetic polymorphisms in DRD2 (rs6275 and rs6276) and ANKK1 (rs1800497) are associated with bruxism in construction men workers. A total of 113 male patients were evaluated. Bruxism was determined using a questionnaire, in which the patient self-reported the presence or absence of bruxism. For genetic analysis, saliva was collected from all individuals and the extraction of genomic DNA was performed to investigate the genetic polymorphisms rs6275 (C/T), rs6276 (A/G) and rs1800497 (C/T). The statistical significance was determined adopting an alpha = 0.05.Results Twenty-three (20.35%) patients reported at least one symptom of bruxism. Clenching was reported by 15.93% of the patients and grinding was reported by 14.16% of the patients. There was no statistical significance association between the studied genetic polymorphisms and bruxism (p > .05).Conclusions Our study did not observe an association between the genetic polymorphisms in DRD2 and ANKK1 and bruxism in a group of male construction workers.

Published

2024

4. 锚蛋白重复序列22（ANKRD22）对人肝癌细胞的影响及其机制.

Author

蔡浚哲, 刘松柏, 费晓斌, 刘 鹏, 朱昌毫, 王 兴, and 潘耀振

Abstract

Objective To investigate the effect of ankyrin-repeat domain-containing protein 22 (ANKRD22) on the proliferation, invasion, and migration of human hepatoma cells and its molecular mechanism. Methods The TCGA database was used to analyze the expression level of ANKRD22 in normal liver tissue and hepatocellular carcinoma tissue and its association with prognosis. Western Blot and qRT-PCR were used to measure the expression of ANKRD22 in human normal liver cells (L-02) and human hepatoma cells (Huh7, HepG2, MHCC-97H, SK-HEP-1, and SMMC-7721); CCK-8 assay, EdU, wound healing assay, and Transwell assay were used to observe the effect of ANKRD22 on the proliferation, invasion, and migration of hepatoma cells; Western Blot was used to investigate the association of ANKRD22 with cyclins and EMTrelated proteins; KEGG and ssGSEA analyses were performed to investigate the mechanism of action of ANKRD22 in hepatoma cells, and related experiments were conducted for validation. The independent-samples t-test was used for comparison of continuous data between two groups; a one-way analysis of variance was used for comparison between multiple groups, and the least significant difference t-test was used for further comparison between two groups. Results In the TCGA database, the expression level of ANKRD22 in hepatoma tissue was significantly higher than that in normal liver tissue (t= 5.083, P<0.05), and the patients with a high expression level of ANKRD22 had longer overall survival and disease-related survival than those with a low expression level of ANKRD22 (P<0.05). The expression level of ANKRD22 in various human hepatoma cell lines was higher than that in human normal liver cells (all P<0.05). Cell proliferation assay showed that the ANKRD22 overexpression group had significantly higher EdU positive rate and proliferation rate than the Vector group (t= 19.60 and 6.72, both P<0.001), and compared with the si-NC group, the si-ANKRD22#2 group and the si-ANKRD22#3 group had significantly lower EdU positive rate and proliferation rate (all P<0.001). Compared with the Vector group, the overexpression group had significantly higher expression levels of Cyclin E1, Cyclin D1, CDK7, and CDK4 (t=3.54, 4.95, 6.34, and 5.19, all P<0.01), and the si-ANKRD22#2 group and the si-ANKRD22#3 group had significantly lower expression levels than the si-NC group (all P<0.001). The overexpression group had a significantly lower expression level of P27 than the Vector group (t=6.12, P<0.001), and the si-ANKRD22#2 group and the si-ANKRD22#3 group had a significantly higher expression level than the si-NC group (both P<0.001). Invasion and migration experiments showed that compared with the Vector group, the ANKRD22 overexpression group had significantly higher migration rate and number of crossings through the membrane (migration group and invasion group) (t=5.01, 25.60, and 3.67, all P<0.05), and compared with the si-NC group, thesi-ANKRD22#2 group and the si-ANKRD22#3 group had significantly lower migration rate and number of crossings through the membrane (migration group and invasion group) (all P<0.01). The overexpression group had significantly higher expression levels of N-cadherin, Vimentin, and Snail than the Vector group (t=12.13, 8.85, and 13.97, all P<0.001), and the si-ANKRD22#2 group and the si-ANKRD22#3 group had significantly lower expression levels than the si-NC group (all P< 0.001); the overexpression group had a significantly lower expression level of E-cadherin than the Vector group (t=4.98, P< 0.01), and the si-ANKRD22#2 group and the si-ANKRD22#3 group had a significantly higher expression level than the si-NC group (both P<0.001). The KEGG enrichment analysis and the ssGSEA analysis showed that ANKRD22 was associated with the PI3K/AKT/mTOR signaling pathway in hepatocellular carcinoma, and the overexpression group had significantly higher expression levels of p-AKT/AKT, p-PI3K/PI3K, and p-mTOR/mTOR than the Vector group (t=12.21, 3.43, and 9.75, all P< 0.01), and the si-ANKRD22#2 group and the si-ANKRD22#3 group had significantly lower expression levels than the si-NC group (all P<0.001). Conclusion ANKRD22 is highly expressed in hepatoma cells and can promote the proliferation, invasion, and migration of hepatoma cells and the activation of the PI3K/AKT/mTOR signaling pathway. [ABSTRACT FROM AUTHOR]

Published

2024

5. Structure, dynamics and assembly of the ankyrin complex on human red blood cell membrane

Author

Xia, Xian, Liu, Shiheng, and Zhou, Z Hong

Subjects

Biochemistry and Cell Biology, Biological Sciences, Rare Diseases, Hematology, Underpinning research, 1.1 Normal biological development and functioning, Aetiology, 2.1 Biological and endogenous factors, Generic health relevance, Ankyrin Repeat, Ankyrins, Cryoelectron Microscopy, Cytoskeleton, Erythrocyte Membrane, Humans, Chemical Sciences, Medical and Health Sciences, Biophysics, Developmental Biology, Biological sciences, Biomedical and clinical sciences, Chemical sciences

Abstract

The cytoskeleton of a red blood cell (RBC) is anchored to the cell membrane by the ankyrin complex. This complex is assembled during RBC genesis and comprises primarily band 3, protein 4.2 and ankyrin, whose mutations contribute to numerous human inherited diseases. High-resolution structures of the ankyrin complex have been long sought-after to understand its assembly and disease-causing mutations. Here, we analyzed native complexes on the human RBC membrane by stepwise fractionation. Cryo-electron microscopy structures of nine band-3-associated complexes reveal that protein 4.2 stabilizes the cytoplasmic domain of band 3 dimer. In turn, the superhelix-shaped ankyrin binds to this protein 4.2 via ankyrin repeats (ARs) 6-13 and to another band 3 dimer via ARs 17-20, bridging two band 3 dimers in the ankyrin complex. Integration of these structures with both prior data and our biochemical data supports a model of ankyrin complex assembly during erythropoiesis and identifies interactions essential for the mechanical stability of RBC.

Published

2022

6. ASAP1 Expression in Invasive Breast Cancer and Its Prognostic Role.

Author

Park, Hosub, Son, Hwangkyu, Cha, Hyebin, Song, Kihyuk, Bang, Seongsik, Jee, Seungyun, Kim, Hyunsung, Myung, Jaekyung, Shin, Su-Jin, Cha, Chihwan, Chung, Min Sung, and Paik, Seungsam

Subjects

*CANCER invasiveness, *BREAST cancer, *PROGRESSION-free survival, *IMMUNOSTAINING, *OVERALL survival, *SURVIVAL analysis (Biometry), *MULTIVARIATE analysis, *BREAST

Abstract

Breast cancer is a major global health burden with high morbidity and mortality rates. Previous studies have reported that increased expression of ASAP1 is associated with poor prognosis in various types of cancer. This study was conducted on 452 breast cancer patients who underwent surgery at Hanyang University Hospital, Seoul, South Korea. Data on clinicopathological characteristics including molecular pathologic markers were collected. Immunohistochemical staining of ASAP1 expression level were used to classify patients into high and low groups. In total, 452 cases low ASAP1 expression group was associated with significantly worse recurrence-free survival (p = 0.029). In ER-positive cases (n = 280), the low ASAP1 expression group was associated with significantly worse overall survival (p = 0.039) and recurrence-free survival (p = 0.029). In multivariate cox analysis, low ASAP1 expression was an independent significant predictor of poor recurrence-free survival in the overall patient group (hazard ratio = 2.566, p = 0.002) and ER-positive cases (hazard ratio = 4.046, p = 0.002). In the analysis of the TCGA dataset, the low-expression group of ASAP1 protein demonstrated a significantly poorer progression-free survival (p = 0.005). This study reports that low ASAP1 expression was associated with worse recurrence-free survival in invasive breast cancer. [ABSTRACT FROM AUTHOR]

Published

2023

7. Ankyrin2 is essential for neuronal morphogenesis and long-term courtship memory in Drosophila

Author

Silvia Schwartz, Sarah J Wilson, Tracy K Hale, and Helen L Fitzsimons

Subjects

Ankyrin repeat, Ankyrin2, ANK3, Histone deacetylase, HDAC4, Memory, Neurology. Diseases of the nervous system, RC346-429

Abstract

Abstract Dysregulation of HDAC4 expression and/or nucleocytoplasmic shuttling results in impaired neuronal morphogenesis and long-term memory in Drosophila melanogaster. A recent genetic screen for genes that interact in the same molecular pathway as HDAC4 identified the cytoskeletal adapter Ankyrin2 (Ank2). Here we sought to investigate the role of Ank2 in neuronal morphogenesis, learning and memory. We found that Ank2 is expressed widely throughout the Drosophila brain where it localizes predominantly to axon tracts. Pan-neuronal knockdown of Ank2 in the mushroom body, a region critical for memory formation, resulted in defects in axon morphogenesis. Similarly, reduction of Ank2 in lobular plate tangential neurons of the optic lobe disrupted dendritic branching and arborization. Conditional knockdown of Ank2 in the mushroom body of adult Drosophila significantly impaired long-term memory (LTM) of courtship suppression, and its expression was essential in the γ neurons of the mushroom body for normal LTM. In summary, we provide the first characterization of the expression pattern of Ank2 in the adult Drosophila brain and demonstrate that Ank2 is critical for morphogenesis of the mushroom body and for the molecular processes required in the adult brain for the formation of long-term memories.

Published

2023

8. Developing nanobodies to stabilise the tumour suppressor protein p16INK4a

Author

Burbidge, Owen David and Itzhaki, Laura

Subjects

616.99, heavy-chain antibody, antibody, nanobody, tumour suppressor, p16ink4a, cdkn2a, p16, camelid, crystallography, biophysics, protein stability, ankyrin repeat, cell-cycle control

Abstract

The tumour suppressor protein p16INK4a (p16) is a cyclin-dependent kinase (CDK) inhibitor that plays a key role in the regulation of the cell cycle by controlling the progression of cells through the G1 to S phase transition. Dysregulation of the protein through deletion, silencing or mutation of the gene encoding p16 is implicated in a range of different cancers including melanoma, cervical and oesophageal to name a few. p16 is composed of four ankyrin repeats and it has a very low thermodynamic and kinetic stability and rapidly unfolds even in the absence of denaturants. This low stability means that the protein is highly vulnerable to point mutations, which can result in functional inactivation through a range of different mechanisms such as deletion of key binding contacts, disruption of secondary or tertiary structure and consequent destabilisation leading to unfolding or aggregation. Heavy-chain antibodies are a unique form of antibody devoid of light chains found in the serum of the Camelid family (camels and llamas). Despite the absence of light chains, heavy-chain antibodies have evolved to complement traditional antibodies and retain the full binding capacity seen in canonical IgG antibodies. The single variable domain, known as a nanobody, is, at 15 kDa, the smallest antigen binding fragment, a tenth the size of a standard IgG antibody. The small size and relative ease of production, coupled with an unusually high stability, makes nanobodies useful tools as biological reagents, crystallography chaperones and therapeutics. The research contained within this PhD looks at the development of nanobodies to target p16. By leveraging the high stability of selected nanobodies, the aim was to obtain binders that could stabilise and reactivate a range of unstable cancer-associated mutants. The initial stages of the project focused on generating and optimising the expression and purification of p16 constructs prior to immunisation of animals to raise nanobodies. A high-throughput approach was taken to generate forty-five different p16 constructs with a range of different solubility and purification tags. These constructs were assessed in a multi-factorial expression screen, which resulted in the identification of a p16 construct with a ten-fold improvement in soluble expression levels compared with previous studies. A range of biophysical techniques, including circular dichroism and chemical denaturation, were performed to characterise this protein fully prior to immunisation. The second part of this project utilised a phage display library of two immune nanobody libraries generated against p16 and a p16 variant stabilised by previously published second-site mutations. This process yielded a large number of diverse nanobodies. Biophysical characterisation of these nanobodies was first performed, and they were found to have a range of chemical and thermal stabilities. Assays were then developed to test the ability of the nanobodies to stabilise p16. Two nanobodies were found to dramatically stabilise wild-type p16, with an increase in stability of approximately 44 % and 60 %, respectively. Furthermore, these nanobodies were also able to stabilise a subset of cancer-associated point mutants. Although there are NMR structures of p16, as well as a crystal structure of p16 bound to CDK6, the resolution of is very low, most likely due to the high backbone flexibility of p16. The last part of the project aimed to obtain a higher-resolution structure of p16 by using the two stabilising nanobodies as crystallisation chaperones. The more stabilising of the two nanobodies resulted in crystals that diffracted to a resolution of less than 2 $\AA$, a significant improvement compared with the previously published structure. In conclusion, a number of nanobodies were generated against tumour-associated p16 and shown to be capable of stabilising p16, allowing structure determination to high resolution and restoration of the stability of cancer-associated mutants to wild-type levels. In the project, a range of different approaches for nanobody production were explored, and these will be important for future applications. Moreover, the crystal structure of the p16-nanobody complex showed that the nanobody binds on the opposite face of p16, to the face involved in binding to CDKs; thus, this nanobody could potentially be exploited as a pharmacological chaperone to stabilise and restore the activity of cancer-associated mutant p16 in the cell.

Published

2019

9. Ankyrin2 is essential for neuronal morphogenesis and long-term courtship memory in Drosophila.

Author

Schwartz, Silvia, Wilson, Sarah J, Hale, Tracy K, and Fitzsimons, Helen L

Subjects

*LONG-term memory, *ANIMAL courtship, *NUCLEOCYTOPLASMIC interactions, *DROSOPHILA melanogaster, *GENETIC testing, *MORPHOGENESIS

Abstract

Dysregulation of HDAC4 expression and/or nucleocytoplasmic shuttling results in impaired neuronal morphogenesis and long-term memory in Drosophila melanogaster. A recent genetic screen for genes that interact in the same molecular pathway as HDAC4 identified the cytoskeletal adapter Ankyrin2 (Ank2). Here we sought to investigate the role of Ank2 in neuronal morphogenesis, learning and memory. We found that Ank2 is expressed widely throughout the Drosophila brain where it localizes predominantly to axon tracts. Pan-neuronal knockdown of Ank2 in the mushroom body, a region critical for memory formation, resulted in defects in axon morphogenesis. Similarly, reduction of Ank2 in lobular plate tangential neurons of the optic lobe disrupted dendritic branching and arborization. Conditional knockdown of Ank2 in the mushroom body of adult Drosophila significantly impaired long-term memory (LTM) of courtship suppression, and its expression was essential in the γ neurons of the mushroom body for normal LTM. In summary, we provide the first characterization of the expression pattern of Ank2 in the adult Drosophila brain and demonstrate that Ank2 is critical for morphogenesis of the mushroom body and for the molecular processes required in the adult brain for the formation of long-term memories. [ABSTRACT FROM AUTHOR]

Published

2023

10. Computational design of a modular protein sense-response system

Author

Glasgow, Anum A, Huang, Yao-Ming, Mandell, Daniel J, Thompson, Michael, Ritterson, Ryan, Loshbaugh, Amanda L, Pellegrino, Jenna, Krivacic, Cody, Pache, Roland A, Barlow, Kyle A, Ollikainen, Noah, Jeon, Deborah, Kelly, Mark JS, Fraser, James S, and Kortemme, Tanja

Subjects

Information and Computing Sciences, Biochemistry and Cell Biology, Biological Sciences, Bioengineering, Biotechnology, Generic health relevance, Ankyrin Repeat, Binding Sites, Biosensing Techniques, Computational Biology, Computer Simulation, Crystallography, X-Ray, Ligands, Maltose-Binding Proteins, Models, Molecular, Polyisoprenyl Phosphates, Protein Engineering, Protein Multimerization, Proteins, Sesquiterpenes, General Science & Technology

Abstract

Sensing and responding to signals is a fundamental ability of living systems, but despite substantial progress in the computational design of new protein structures, there is no general approach for engineering arbitrary new protein sensors. Here, we describe a generalizable computational strategy for designing sensor-actuator proteins by building binding sites de novo into heterodimeric protein-protein interfaces and coupling ligand sensing to modular actuation through split reporters. Using this approach, we designed protein sensors that respond to farnesyl pyrophosphate, a metabolic intermediate in the production of valuable compounds. The sensors are functional in vitro and in cells, and the crystal structure of the engineered binding site closely matches the design model. Our computational design strategy opens broad avenues to link biological outputs to new signals.

Published

2019

11. Hypermethylated gene ANKDD1A is a candidate tumor suppressor that interacts with FIH1 and decreases HIF1α stability to inhibit cell autophagy in the glioblastoma multiforme hypoxia microenvironment

Author

Feng, Jianbo, Zhang, Yan, She, Xiaoling, Sun, Yingnan, Fan, Li, Ren, Xing, Fu, Haijuan, Liu, Changhong, Li, Peiyao, Zhao, Chunhua, Liu, Qiang, Liu, Qing, Li, Guiyuan, and Wu, Minghua

Subjects

Biomedical and Clinical Sciences, Oncology and Carcinogenesis, Brain Disorders, Genetics, Rare Diseases, Neurosciences, Cancer, Orphan Drug, Brain Cancer, 2.1 Biological and endogenous factors, Aetiology, Ankyrin Repeat, Apoptosis, Autophagy, Cell Line, Tumor, Chromosomes, Human, Pair 15, DNA Methylation, Gene Expression Regulation, Neoplastic, Genes, Tumor Suppressor, Glioblastoma, Glucose, Half-Life, Humans, Hypoxia-Inducible Factor 1, alpha Subunit, Intracellular Signaling Peptides and Proteins, Lactates, Mixed Function Oxygenases, Neoplasm Proteins, Protein Stability, Recombinant Proteins, Repressor Proteins, Transcription, Genetic, Tumor Hypoxia, Tumor Microenvironment, Tumor Suppressor Proteins, Up-Regulation, Von Hippel-Lindau Tumor Suppressor Protein, Clinical Sciences, Oncology & Carcinogenesis, Biochemistry and cell biology, Oncology and carcinogenesis

Abstract

Ectopic epigenetic mechanisms play important roles in facilitating tumorigenesis. Here, we first demonstrated that ANKDD1A is a functional tumor suppressor gene, especially in the hypoxia microenvironment. ANKDD1A directly interacts with FIH1 and inhibits the transcriptional activity of HIF1α by upregulating FIH1. In addition, ANKDD1A decreases the half-life of HIF1α by upregulating FIH1, decreases glucose uptake and lactate production, inhibits glioblastoma multiforme (GBM) autophagy, and induces apoptosis in GBM cells under hypoxia. Moreover, ANKDD1A is highly frequently methylated in GBM. The tumor-specific methylation of ANKDD1A indicates that it could be used as a potential epigenetic biomarker as well as a possible therapeutic target.

Published

2019

12. Snapshots of urea‐induced early structural changes and unfolding of an ankyrin repeat protein at atomic resolution.

Author

Medur Gurushankar, Mukund Sudharsan, Dalvi, Somavally, and Venkatraman, Prasanna

Abstract

Protein folding and unfolding is a complex process, underscored by the many proteotoxic diseases associated with misfolded proteins. Mapping pathways from a native structure to an unfolded protein or vice versa, identifying the intermediates, and defining the role of sequence and structure en route remain outstanding problems in the field. It is even more challenging to capture the events at atomistic resolution. X‐ray diffraction has so far been used to understand how urea interacts with and unfolds two stable globular proteins. Here, we present the case study on PSMD10Gankyrin, a prototype for a moderately stable, non‐globular repeat protein, long and rigid, with its termini located at either end. We define structural changes in the time dimension using low urea concentrations to arrive at the following conclusions. (a) Unfolding is rapidly initiated at the C‐terminus, slowly at the N‐terminus, and proceeds inwards from both ends. (b) C‐terminus undergoes an α to 310 helix transition, representing the structure of a potential early unfolding intermediate before disorder sets in. (c) Distinct and progressive changes in the electrostatic landscape of PSMD10Gankyrin were observed, indicative of conformational changes in the seemingly inflexible motif involved in protein–protein interaction. We believe this unique study will open up the field for better and bolder queries and increase the choice of model proteins for a better understanding of the challenging problems of protein folding, protein interactions, protein degradation, and diseases associated with misfolding. PDB Code(s): 7VXV, 7VXW, 7VY4 and 7VY7; [ABSTRACT FROM AUTHOR]

Published

2022

13. ASAP1 Expression in Invasive Breast Cancer and Its Prognostic Role

Author

Hosub Park, Hwangkyu Son, Hyebin Cha, Kihyuk Song, Seongsik Bang, Seungyun Jee, Hyunsung Kim, Jaekyung Myung, Su-Jin Shin, Chihwan Cha, Min Sung Chung, and Seungsam Paik

Subjects

ArfGAP with SH3 domain, ankyrin repeat, PH domain 1, invasive breast carcinoma, prognosis, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

Breast cancer is a major global health burden with high morbidity and mortality rates. Previous studies have reported that increased expression of ASAP1 is associated with poor prognosis in various types of cancer. This study was conducted on 452 breast cancer patients who underwent surgery at Hanyang University Hospital, Seoul, South Korea. Data on clinicopathological characteristics including molecular pathologic markers were collected. Immunohistochemical staining of ASAP1 expression level were used to classify patients into high and low groups. In total, 452 cases low ASAP1 expression group was associated with significantly worse recurrence-free survival (p = 0.029). In ER-positive cases (n = 280), the low ASAP1 expression group was associated with significantly worse overall survival (p = 0.039) and recurrence-free survival (p = 0.029). In multivariate cox analysis, low ASAP1 expression was an independent significant predictor of poor recurrence-free survival in the overall patient group (hazard ratio = 2.566, p = 0.002) and ER-positive cases (hazard ratio = 4.046, p = 0.002). In the analysis of the TCGA dataset, the low-expression group of ASAP1 protein demonstrated a significantly poorer progression-free survival (p = 0.005). This study reports that low ASAP1 expression was associated with worse recurrence-free survival in invasive breast cancer.

Published

2023

14. Structural Basis of Activity of HER2-Targeting Construct Composed of DARPin G3 and Albumin-Binding Domains.

Author

Konshina AG, Bocharov EV, Konovalova EV, Schulga AA, Tolmachev V, Deyev SM, and Efremov RG

Subjects

Humans, Binding Sites, Models, Molecular, Ankyrin Repeat, Recombinant Fusion Proteins metabolism, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Protein Domains, Receptor, ErbB-2 metabolism, Receptor, ErbB-2 chemistry, Protein Binding

Abstract

Non-immunoglobulin-based scaffold proteins (SPs) represent one of the key therapeutic target-specific and high-affinity binders in modern medicine. Among their cellular targets are signaling receptors, in particular, receptor tyrosine kinases, whose dysfunction leads to the development of cancer and other serious diseases. Successful applications of SPs have been reported for HER receptor type 2 (HER2), a member of the human epidermal growth factor receptor family that regulates cell growth and differentiation. To extend the blood residence of SPs and prevent their high accumulation in the kidneys, these proteins are often fused with serum albumin. Promising results for HER2-binding activity were obtained for SP G3 from the DARPins (Designed Ankyrin Repeat Proteins) family fused with an albumin-binding domain (ABD). Interestingly, the detected HER2-G3 binding strongly depended on the position of the G3 module in the sequence of the constructs. Further improvement of these constructs for biomedical applications requires deciphering the molecular mechanism responsible for this effect. Here, we investigate the structural and dynamic aspects of ABD-G3 and G3-ABD chimeras using NMR spectroscopy and molecular modeling. Based on biophysical data, we come to the conclusion that extensive inter-domain contacts form in both constructs, although their binding interfaces and complex stability are somewhat different. Also, it is shown that the domain linker plays an important role-it limits the accessibility of the detected protein-protein binding sites, depending on the order of the domains in the chimeric molecules. These results create a solid structural basis for the rational design of new effective SP constructs targeting the signaling receptors in cells.

Published

2024

15. crANKing up the infection: ankyrin domains in Rickettsiales and their role in host manipulation.

Author

Hamilton WC and Newton ILG

Subjects

Humans, Animals, Ankyrin Repeat, Rickettsiaceae genetics, Rickettsiaceae metabolism, Host-Pathogen Interactions, Bacterial Proteins metabolism, Bacterial Proteins genetics

Abstract

Intracellular bacteria use secreted effector proteins to modify host biology and facilitate infection. For many of these microbes, a particular eukaryotic domain-the ankyrin repeat (ANK)-plays a central role in specifying the host proteins and pathways targeted by the microbe. While we understand much of how some ANKs function in model organisms like Legionella and Coxiella , the understudied Rickettsiales species harbor many proteins with ANKs, some of which play critical roles during infection. This minireview is meant to organize and summarize the research progress made in understanding some of these Rickettsiales ANKs as well as document some of the techniques that have driven much of this progress., Competing Interests: The authors declare no conflict of interest.

Published

2024

16. Dimerization activates the Inversin complex in C. elegans .

Author

Beyrent E, Wei DT, Beacham GM, Park S, Zheng J, Paszek MJ, and Hollopeter G

Subjects

Animals, Protein Multimerization, Optogenetics methods, Ankyrin Repeat, Dimerization, Phenotype, Protein Serine-Threonine Kinases metabolism, Protein Serine-Threonine Kinases genetics, Caenorhabditis elegans metabolism, Caenorhabditis elegans Proteins metabolism, Caenorhabditis elegans Proteins genetics

Abstract

Genetic, colocalization, and biochemical studies suggest that the ankyrin repeat-containing proteins Inversin (INVS) and ANKS6 function with the NEK8 kinase to control tissue patterning and maintain organ physiology. It is unknown whether these three proteins assemble into a static "Inversin complex" or one that adopts multiple bioactive forms. Through the characterization of hyperactive alleles in C. elegans , we discovered that the Inversin complex is activated by dimerization. Genome engineering of an RFP tag onto the nematode homologues of INVS (MLT-4) and NEK8 (NEKL-2) induced a gain-of-function, cyst-like phenotype that was suppressed by monomerization of the fluorescent tag. Stimulated dimerization of MLT-4 or NEKL-2 using optogenetics was sufficient to recapitulate the phenotype of a constitutively active Inversin complex. Further, dimerization of NEKL-2 bypassed a lethal MLT-4 mutant, demonstrating that the dimeric form is required for function. We propose that dynamic switching between at least two functionally distinct states - an active dimer and an inactive monomer - gates the output of the Inversin complex., Competing Interests: Conflicts of interest: The authors declare no competing interest.

Published

2024

17. Deletion of Asb15b gene can lead to a significant decrease in zebrafish intermuscular bone.

Author

Niu M, Whang H, Wu Z, Jiang S, and Chen L

Subjects

Animals, Bone and Bones metabolism, Bone Development genetics, CRISPR-Cas Systems, Gene Deletion, Gene Expression Regulation, Developmental, Muscle, Skeletal metabolism, Ankyrin Repeat, Zebrafish genetics, Zebrafish Proteins genetics, Zebrafish Proteins metabolism

Abstract

Intermuscular bones, which are present in numerous economically significant fish species, have a negative impact on the development of aquaculture. The Asb15b gene, primarily expressed in skeletal muscle, plays a crucial role in regulating protein turnover and the development of muscle fibers. It stimulates protein synthesis and controls the differentiation of muscle fibers. In this study, we employed CRISPR/Cas9 technology to generate homozygous zebrafish strains with 7 bp and 49 bp deletions in the Asb15b gene. Subsequent analyses using skeleton staining demonstrated a substantial reduction in the number of intermuscular bones in adult Asb15b -/- -7 bp and Asb15b -/- -49 bp mutants compared to the wild-type zebrafish, with decreases of 30 % (P < 0.001) and 40 % (P < 0.0001), respectively. Histological experiments further revealed that the diameter and number of muscle fibers in adult Asb15b -/- mutants did not exhibit significant changes when compared to wild-type zebrafish. Moreover, qRT-PCR experiments demonstrated significant differences in the expression of bmp6 and runx2b genes, which are key regulators of intermuscular bone development, during different stages of intermuscular bone development in Asb15b -/- mutants. This study strongly suggests that the Asb15b gene plays a crucial role in regulating intermuscular bone development in fish and lays the groundwork for further exploration of the role of the Asb15b gene in zebrafish intermuscular bone development., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

18. An N-terminal and ankyrin repeat domain interactome of Shank3 identifies the protein complex with the splicing regulator Nono in mice.

Author

Okuzono S, Fujii F, Setoyama D, Taira R, Shinmyo Y, Kato H, Masuda K, Yonemoto K, Akamine S, Matsushita Y, Motomura Y, Sakurai T, Kawasaki H, Han K, Kato TA, Torisu H, Kang D, Nakabeppu Y, Ohga S, and Sakai Y

Subjects

Animals, Mice, Ankyrin Repeat, DNA-Binding Proteins metabolism, DNA-Binding Proteins genetics, Microfilament Proteins metabolism, Microfilament Proteins genetics, RNA Splicing, Brain metabolism, Seizures metabolism, Seizures genetics, Seizures chemically induced, Humans, Protein Binding, Mice, Inbred C57BL, Nerve Tissue Proteins metabolism, Nerve Tissue Proteins genetics, RNA-Binding Proteins metabolism, RNA-Binding Proteins genetics, Mice, Knockout

Abstract

An autism-associated gene Shank3 encodes multiple splicing isoforms, Shank3a-f. We have recently reported that Shank3a/b-knockout mice were more susceptible to kainic acid-induced seizures than wild-type mice at 4 weeks of age. Little is known, however, about how the N-terminal and ankyrin repeat domains (NT-Ank) of Shank3a/b regulate multiple molecular signals in the developing brain. To explore the functional roles of Shank3a/b, we performed a mass spectrometry-based proteomic search for proteins interacting with GFP-tagged NT-Ank. In this study, NT-Ank was predicted to form a variety of complexes with a total of 348 proteins, in which RNA-binding (n = 102), spliceosome (n = 22), and ribosome-associated molecules (n = 9) were significantly enriched. Among them, an X-linked intellectual disability-associated protein, Nono, was identified as a NT-Ank-binding protein. Coimmunoprecipitation assays validated the interaction of Shank3 with Nono in the mouse brain. In agreement with these data, the thalamus of Shank3a/b-knockout mice aberrantly expressed splicing isoforms of autism-associated genes, Nrxn1 and Eif4G1, before and after seizures with kainic acid treatment. These data indicate that Shank3 interacts with multiple RNA-binding proteins in the postnatal brain, thereby regulating the homeostatic expression of splicing isoforms for autism-associated genes after birth., (© 2024 The Author(s). Genes to Cells published by Molecular Biology Society of Japan and John Wiley & Sons Australia, Ltd.)

Published

2024

19. Myosin XVI

Author

Bugyi, Beáta, Kengyel, András, Crusio, Wim E., Series Editor, Lambris, John D., Series Editor, Radeke, Heinfried H., Series Editor, Rezaei, Nima, Series Editor, and Coluccio, Lynne M., editor

Published

2020

20. Discovery and Analysis of Repeat and Low-Complexity Architectures in Proteins and Their Conserved Evolutionary Relationships Using Self-Homology Dot Plots.

Author

Górna MW and Merski M

Subjects

Conserved Sequence, Repetitive Sequences, Amino Acid, Computational Biology methods, Amino Acid Sequence, Databases, Protein, Cluster Analysis, Software, Sequence Analysis, Protein methods, Proteins chemistry, Proteins genetics, Evolution, Molecular

Abstract

Proteins that contain sequence repetitions and low complexity regions can be analyzed using self-homology dot plot analysis. Dot plots can readily identify protein sequence repeats; the number of repeats and their length and location within the protein sequence are readily identifiable from the dot plots without the need to pre-define any of these attributes, making this method largely model-independent. We discuss the criteria for statistical identification of protein repeats and recommend simple ways of identifying protein repeats. While higher levels of sequence conservation within the repeats do make them easier to formally identify, this method can identify protein repeats with fairly low levels of conservation, as well as notably non-tandem repetitions with sizeable sections of complex, non-repeat sequence separating the individual repeat instances. Furthermore, even simple visual examination of these dot plots can discover conserved patterns within families of closely related proteins, and the level of this conservation can be readily quantified using a Jaccard index. Exhaustive pairwise comparisons can be assembled using hierarchical clustering methods to get a picture of the conserved repeat architectures within families of repeat proteins., (© 2025. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2025

21. Comparative Genomics of a Parthenogenesis-Inducing Wolbachia Symbiont.

Author

Lindsey, Amelia RI, Werren, John H, Richards, Stephen, and Stouthamer, Richard

Subjects

Animals, Culicidae, Drosophila, Wasps, Wolbachia, Bacterial Proteins, Genomics, Phylogeny, Symbiosis, Ankyrin Repeat, Parthenogenesis, Frameshift Mutation, Genome, Bacterial, Open Reading Frames, Biological Evolution, Host Specificity, Rickettsiales, Trichogramma, gene truncations, genome content, symbiosis, Genome, Bacterial, Genetics

Abstract

Wolbachia is an intracellular symbiont of invertebrates responsible for inducing a wide variety of phenotypes in its host. These host-Wolbachia relationships span the continuum from reproductive parasitism to obligate mutualism, and provide a unique system to study genomic changes associated with the evolution of symbiosis. We present the genome sequence from a parthenogenesis-inducing Wolbachia strain (wTpre) infecting the minute parasitoid wasp Trichogramma pretiosum The wTpre genome is the most complete parthenogenesis-inducing Wolbachia genome available to date. We used comparative genomics across 16 Wolbachia strains, representing five supergroups, to identify a core Wolbachia genome of 496 sets of orthologous genes. Only 14 of these sets are unique to Wolbachia when compared to other bacteria from the Rickettsiales. We show that the B supergroup of Wolbachia, of which wTpre is a member, contains a significantly higher number of ankyrin repeat-containing genes than other supergroups. In the wTpre genome, there is evidence for truncation of the protein coding sequences in 20% of ORFs, mostly as a result of frameshift mutations. The wTpre strain represents a conversion from cytoplasmic incompatibility to a parthenogenesis-inducing lifestyle, and is required for reproduction in the Trichogramma host it infects. We hypothesize that the large number of coding frame truncations has accompanied the change in reproductive mode of the wTpre strain.

Published

2016

22. Binding of NFκB Appears to Twist the Ankyrin Repeat Domain of IκBα

Author

Trelle, Morten Beck, Ramsey, Kristen M, Lee, Taehyung C, Zheng, Weihua, Lamboy, Jorge, Wolynes, Peter G, Deniz, Ashok, and Komives, Elizabeth A

Subjects

Biological Sciences, Chemical Sciences, Physical Chemistry, Underpinning research, 1.1 Normal biological development and functioning, Amides, Ankyrin Repeat, Molecular Dynamics Simulation, NF-KappaB Inhibitor alpha, NF-kappa B, Protein Binding, Physical Sciences, Biophysics, Biological sciences, Chemical sciences, Physical sciences

Abstract

Total internal reflection fluorescence-based single-molecule Förster resonance energy transfer (FRET) measurements were previously carried out on the ankyrin repeat domain (ARD) of IκBα, the temporally regulated inhibitor of canonical NFκB signaling. Under native conditions, most of the IκBα molecules showed stable, high FRET signals consistent with distances between the fluorophores estimated from the crystal structures of the NFκB(RelA/p50)-IκBα complex. Similar high FRET efficiencies were found when the IκBα molecules were either free or in complex with NFκB(RelA/p50), and were interpreted as being consistent with the crystallographically observed ARD structure. An exception to this was observed when the donor and acceptor fluorophores were attached in AR3 (residue 166) and AR6 (residue 262). Surprisingly, the FRET efficiency was lower for the bound IκBα molecules (0.67) than for the free IκBα molecules (0.74), apparently indicating that binding of NFκB(RelA/p50) stretches the ARD of IκBα. Here, we conducted confocal-based single-molecule FRET studies to investigate this phenomenon in greater detail. The results not only recapitulated the apparent stretching of the ARD but also showed that the effect was more pronounced when the N-terminal domains (NTDs) of both RelA and p50 were present, even though the interface between NFκB(RelA/p50) and IκBα encompasses only the dimerization domains. We also performed mass spectrometry-detected amide hydrogen/deuterium exchange (HDXMS) experiments on IκBα as well as IκBα bound to dimerization-domain-only constructs or full-length NFκB(RelA/p50). Although we expected the stretched IκBα to have regions with increased exchange, instead the HDXMS experiments showed decreases in exchange in AR3 and AR6 that were more pronounced when the NFκB NTDs were present. Simulations of the interaction recapitulated the increased distance between residues 166 and 262, and also provide a plausible mechanism for a twisting of the IκBα ARD induced by interactions of the IκBα proline-glutamate-serine-threonine-rich sequence with positively charged residues in the RelA NTD.

Published

2016

23. Redesigning amino/carboxyl ends of DARPin G3 for high thermostability and production in tobacco transplastomic plants.

Author

Kohnehrouz BB and Ehsasatvatan M

Subjects

Plant Leaves metabolism, Plant Leaves genetics, Molecular Dynamics Simulation, Hot Temperature, Protein Engineering methods, Nicotiana genetics, Nicotiana metabolism, Protein Stability, Plants, Genetically Modified, Ankyrin Repeat

Abstract

Key Message: Redesigning the N- and C-capping repeats of the native DARPin G3 significantly improved its stability, and may facilitate its purification from the total soluble proteins of high-temperature dried leaf materials of transplastomic plants. Designed ankyrin repeat proteins (DARPins) constitute a promising class of binding molecules that can overcome the limitations of monoclonal antibodies and enable the development of novel therapeutic approaches. Despite their inherent stability, detailed studies have revealed that the original capping repeats derived from natural ankyrin repeat proteins impair the stability of the initial DARPin design. Consequently, the development of thermodynamically stabilized antibody mimetics may facilitate the development of innovative drugs in the future. In this study, we replaced the original N- and C-capping repeats with improved caps to enhance the thermostability of native DARPin G3. Computational analyses suggested that the redesigned thermostable DARPin G3 structure possessed optimal quality and stability. Molecular dynamics simulations verified the stability of the redesigned thermostable DARPin G3 at high temperatures. The redesigned thermostable DARPin G3 was expressed at high levels in tobacco transplastomic plants and subsequently purified from high-temperature dried leaf materials. Thermal denaturation results revealed that the redesigned thermostable DARPin G3 had a higher Tm value than the native DARPin G3, with a Tm of 35.51 °C greater than that of native DARPin G3. The results of the in vitro bioassays confirmed that the purified thermostable DARPin G3 from high-temperature dried leaf materials maintained its binding activity without any loss of affinity and specifically bound to the HER2 receptor on the cell surface. These findings demonstrate the successful improvement in the thermostability of DARPin G3 without compromising its biological activity., (© 2024. The Author(s), under exclusive licence to Springer-Verlag GmbH Germany, part of Springer Nature.)

Published

2024

24. The RXLR effector PpE18 of Phytophthora parasitica is a virulence factor and suppresses peroxisome membrane-associated ascorbate peroxidase NbAPX3-1-mediated plant immunity.

Author

Cao Y, Zhang Q, Liu Y, Yan T, Ding L, Yang Y, Meng Y, and Shan W

Subjects

Plant Diseases microbiology, Plant Diseases immunology, Protein Binding, Disease Resistance, Ankyrin Repeat, Phytophthora pathogenicity, Phytophthora physiology, Plant Immunity, Nicotiana microbiology, Reactive Oxygen Species metabolism, Ascorbate Peroxidases metabolism, Virulence Factors metabolism, Peroxisomes metabolism

Abstract

Phytophthora parasitica causes diseases on a broad range of host plants. It secretes numerous effectors to suppress plant immunity. However, only a few virulence effectors in P. parasitica have been characterized. Here, we highlight that PpE18, a conserved RXLR effector in P. parasitica, was a virulence factor and suppresses Nicotiana benthamiana immunity. Utilizing luciferase complementation, co-immunoprecipitation, and GST pull-down assays, we determined that PpE18 targeted NbAPX3-1, a peroxisome membrane-associated ascorbate peroxidase with reactive oxygen species (ROS)-scavenging activity and positively regulates plant immunity in N. benthamiana. We show that the ROS-scavenging activity of NbAPX3-1 was critical for its immune function and was hindered by the binding of PpE18. The interaction between PpE18 and NbAPX3-1 resulted in an elevation of ROS levels in the peroxisome. Moreover, we discovered that the ankyrin repeat-containing protein NbANKr2 acted as a positive immune regulator, interacting with both NbAPX3-1 and PpE18. NbANKr2 was required for NbAPX3-1-mediated disease resistance. PpE18 competitively interfered with the interaction between NbAPX3-1 and NbANKr2, thereby weakening plant resistance. Our results reveal an effective counter-defense mechanism by which P. parasitica employed effector PpE18 to suppress host cellular defense, by suppressing biochemical activity and disturbing immune function of NbAPX3-1 during infection., (© 2024 The Authors. New Phytologist © 2024 New Phytologist Foundation.)

Published

2024

25. Preclinical evaluation of EpCAM-binding designed ankyrin repeat proteins (DARPins) as targeting moieties for bimodal near-infrared fluorescence and photoacoustic imaging of cancer.

Author

Houvast RD, Badr N, March T, de Muynck LDAN, Sier VQ, Schomann T, Bhairosingh S, Baart VM, Peeters JAHM, van Westen GJP, Plückthun A, Burggraaf J, Kuppen PJK, Vahrmeijer AL, and Sier CFM

Subjects

Humans, Animals, Mice, Cell Line, Tumor, Tissue Distribution, HT29 Cells, Protein Binding, Infrared Rays, Female, Photoacoustic Techniques methods, Ankyrin Repeat, Epithelial Cell Adhesion Molecule metabolism, Optical Imaging methods

Abstract

Purpose: Fluorescence-guided surgery (FGS) can play a key role in improving radical resection rates by assisting surgeons to gain adequate visualization of malignant tissue intraoperatively. Designed ankyrin repeat proteins (DARPins) possess optimal pharmacokinetic and other properties for in vivo imaging. This study aims to evaluate the preclinical potential of epithelial cell adhesion molecule (EpCAM)-binding DARPins as targeting moieties for near-infrared fluorescence (NIRF) and photoacoustic (PA) imaging of cancer., Methods: EpCAM-binding DARPins Ac2, Ec4.1, and non-binding control DARPin Off7 were conjugated to IRDye 800CW and their binding efficacy was evaluated on EpCAM-positive HT-29 and EpCAM-negative COLO-320 human colon cancer cell lines. Thereafter, NIRF and PA imaging of all three conjugates were performed in HT-29&#95;luc2 tumor-bearing mice. At 24 h post-injection, tumors and organs were resected and tracer biodistributions were analyzed., Results: Ac2-800CW and Ec4.1-800CW specifically bound to HT-29 cells, but not to COLO-320 cells. Next, 6 nmol and 24 h were established as the optimal in vivo dose and imaging time point for both DARPin tracers. At 24 h post-injection, mean tumor-to-background ratios of 2.60 ± 0.3 and 3.1 ± 0.3 were observed for Ac2-800CW and Ec4.1-800CW, respectively, allowing clear tumor delineation using the clinical Artemis NIRF imager. Biodistribution analyses in non-neoplastic tissue solely showed high fluorescence signal in the liver and kidney, which reflects the clearance of the DARPin tracers., Conclusion: Our encouraging results show that EpCAM-binding DARPins are a promising class of targeting moieties for pan-carcinoma targeting, providing clear tumor delineation at 24 h post-injection. The work described provides the preclinical foundation for DARPin-based bimodal NIRF/PA imaging of cancer., (© 2023. The Author(s).)

Published

2024

26. ANKZF1 knockdown inhibits glioblastoma progression by promoting intramitochondrial protein aggregation through mitoRQC.

Author

Li G, Wang Z, Gao B, Dai K, Niu X, Li X, Wang Y, Li L, Wu X, Li H, Yu Z, Wang Z, and Chen G

Subjects

Animals, Humans, Mice, Apoptosis, Brain Neoplasms genetics, Brain Neoplasms pathology, Brain Neoplasms metabolism, Cell Line, Tumor, Cell Proliferation, Gene Knockdown Techniques, Unfolded Protein Response, Xenograft Model Antitumor Assays, Ankyrin Repeat, Disease Progression, Glioblastoma pathology, Glioblastoma genetics, Glioblastoma metabolism, Mice, Nude, Mitochondria metabolism, Mitochondria genetics, Mitochondrial Proteins metabolism, Mitochondrial Proteins genetics

Abstract

Protein homeostasis is fundamental to the development of tumors. Ribosome-associated quality-control (RQC) is able to add alanine and threonine to the stagnant polypeptide chain C-terminal (CAT-tail) when protein translation is hindered, while Ankyrin repeat and zinc-finger domain-containing-protein 1 (ANKZF1) can counteract the formation of the CAT-tail, preventing the aggregation of polypeptide chains. In particular, ANKZF1 plays an important role in maintaining mitochondrial protein homeostasis by mitochondrial RQC (mitoRQC) after translation stagnation of precursor proteins targeting mitochondria. However, the role of ANKZF1 in glioblastoma is unclear. Therefore, the current study was aimed to investigate the effects of ANKZF1 in glioblastoma cells and a nude mouse glioblastoma xenograft model. Here, we reported that knockdown of ANKZF1 in glioblastoma cells resulted in the accumulation of CAT-tail in mitochondria, leading to the activated mitochondrial unfolded protein response (UPRmt) and inhibits glioblastoma malignant progression. Excessive CAT-tail sequestered mitochondrial chaperones HSP60, mtHSP70 and proteases LONP1 as well as mitochondrial respiratory chain subunits ND1, Cytb, mtCO2 and ATP6, leading to mitochondrial oxidative phosphorylation dysfunction, membrane potential impairment, and mitochondrial apoptotic pathway activation. Our study highlights ANKZF1 as a valuable target for glioblastoma intervention and provides an innovative insight for the treatment of glioblastoma through the regulating of mitochondrial protein homeostasis., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

27. Molecular characterization and functional analysis of Eimeria tenella ankyrin repeat-containing protein.

Author

Guo H, Zhao Q, Wang H, Zhu S, Dong H, Xie X, Wang L, Chen L, and Han H

Subjects

Animals, Chickens parasitology, Coccidiostats pharmacology, Nitriles pharmacology, Drug Resistance genetics, Coccidiosis parasitology, Coccidiosis veterinary, Poultry Diseases parasitology, Benzamides pharmacology, Lactones, Eimeria tenella genetics, Protozoan Proteins genetics, Protozoan Proteins metabolism, Ankyrin Repeat, Triazines pharmacology

Abstract

Chicken coccidiosis causes disastrous losses to the poultry industry all over the world. Eimeria tenella is the most prevalent of these disease-causing species. Our former RNA-seq indicated that E. tenella ankyrin repeat-containing protein (EtANK) was expressed differently between drug-sensitive (DS) and drug-resistant strains. In this study, we cloned EtANK and analyzed its translational and transcriptional levels using quantitative real-time PCR (qPCR) and western blotting. The data showed that EtANK was significantly upregulated in diclazuril-resistant (DZR) strain and maduramicin-resistant (MRR) strain compared with the drug-sensitive (DS) strain. In addition, the transcription levels in the DZR strains isolated from the field were higher than in the DS strain. The translation levels of EtANK were higher in unsporulated oocysts (UO) than in sporozoites (SZ), sporulated oocysts (SO), or second-generation merozoites (SM), and the protein levels in SM were significantly higher than in UO, SO, and SZ. The results of the indirect immunofluorescence localization showed that the protein was distributed mainly at the anterior region of SZ and on the surface and in the cytoplasm of SM. The fluorescence intensity increased further with its development in vitro. An anti-rEtANK polyclonal antibody inhibited the invasive ability of E. tenella in DF-1 cells. These results showed that EtANK may be related to host cell invasion, required for the parasite's growth in the host, and may be involved in the development of E. tenella resistance to some drugs., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier GmbH. All rights reserved.)

Published

2024

28. A Regulated, Ubiquitin-Independent Degron in IκBα.

Author

Fortmann, Karen T, Lewis, Russell D, Ngo, Kim A, Fagerlund, Riku, and Hoffmann, Alexander

Subjects

Cell Line, 3T3 Cells, Lysosomes, Animals, Humans, Mice, Macrolides, Cycloheximide, Chloroquine, DNA-Binding Proteins, Green Fluorescent Proteins, Ubiquitin, Signal Transduction, Amino Acid Sequence, Ankyrin Repeat, I-kappa B Proteins, Transcription Factor RelA, HEK293 Cells, Proteolysis, NF-KappaB Inhibitor alpha, IκBα, NFκB, degron, protein half-life control, ubiquitin-independent degradation, NF kappa B, I kappa B alpha, Biochemistry & Molecular Biology, Biochemistry and Cell Biology, Medicinal and Biomolecular Chemistry, Microbiology

Abstract

Whereas ubiquitin-dependent degrons have been characterized in some detail, how proteins may be targeted to ubiquitin-independent proteasomal degradation remains unclear. Here we show that IκBα contains an ubiquitin-independent degron whose activity is portable to heterologous proteins such as the globular protein GFP (green fluorescent protein) via a proteasome-dependent, ubiquitin-independent, non-lysosomal pathway. The ubiquitin-independent degradation signal resides in an 11-amino-acid sequence, which is not only sufficient but also required for IκBα's short half-life. Finally, we show that this degron's activity is regulated by the interaction with NFκB, which controls its solvent exposure, and we demonstrate that this regulation of the degron's activity is critical for IκBα's signaling functions.

Published

2015

29. Genome-Wide Association Study of Short-Acting β2-Agonists. A Novel Genome-Wide Significant Locus on Chromosome 2 near ASB3

Author

Israel, Elliot, Lasky-Su, Jessica, Markezich, Amy, Damask, Amy, Szefler, Stanley J, Schuemann, Brooke, Klanderman, Barbara, Sylvia, Jody, Kazani, Shamsah, Wu, Rongling, Martinez, Fernando, Boushey, Homer A, Chinchilli, Vernon M, Mauger, Dave, Weiss, Scott T, and Tantisira, Kelan G

Subjects

Biotechnology, Human Genome, Asthma, Genetics, Lung, 2.1 Biological and endogenous factors, Aetiology, Respiratory, Adrenergic beta-2 Receptor Agonists, Ankyrin Repeat, Bronchodilator Agents, Child, Child, Preschool, Chromosomes, Human, Pair 2, Female, Gene Frequency, Genome-Wide Association Study, Genotyping Techniques, Humans, Male, Muscle, Smooth, Phenotype, Polymorphism, Single Nucleotide, Receptors, Adrenergic, beta-2, Respiratory Mechanics, Suppressor of Cytokine Signaling Proteins, SHARP Investigators, bronchodilator, genotype, single-nucleotide polymorphism, Medical and Health Sciences, Respiratory System

Abstract

Rationaleβ2-Agonists are the most common form of treatment of asthma, but there is significant variability in response to these medications. A significant proportion of this responsiveness may be heritable.ObjectivesTo investigate whether a genome-wide association study (GWAS) could identify novel pharmacogenetic loci in asthma.MethodsWe performed a GWAS of acute bronchodilator response (BDR) to inhaled β2-agonists. A total of 444,088 single-nucleotide polymorphisms (SNPs) were examined in 724 individuals from the SNP Health Association Resource (SHARe) Asthma Resource Project (SHARP). The top 50 SNPs were carried forward to replication in a population of 444 individuals.Measurements and main resultsThe combined P value for four SNPs reached statistical genome-wide significance aftercorrecting for multiple comparisons. Combined P values for rs350729, rs1840321, rs1384918, and rs1319797 were 2.21 × 10(-10), 5.75 × 10(-8), 9.3 × 10(-8), and 3.95 × 10(-8), respectively. The significant variants all map to a novel genetic region on chromosome 2 near the ASB3 gene, a region associated with smooth muscle proliferation. As compared with the wild type, the presence of the minor alleles reduced the degree of BDR by 20% in the original population and by a similar percentage in the confirmatory population.ConclusionsThese GWAS findings for BDR in subjects with asthma suggest that a gene associated with smooth muscle proliferation may influence a proportion of the smooth muscle relaxation that occurs in asthma.

Published

2015

30. Characterization of the SAM domain of the PKD-related protein ANKS6 and its interaction with ANKS3

Author

Leettola, Catherine N, Knight, Mary Jane, Cascio, Duilio, Hoffman, Sigrid, and Bowie, James U

Subjects

Polycystic Kidney Disease, Congenital Structural Anomalies, Kidney Disease, Genetics, Pediatric, 2.1 Biological and endogenous factors, 1.1 Normal biological development and functioning, Aetiology, Underpinning research, Renal and urogenital, Amino Acid Sequence, Animals, Ankyrin Repeat, Binding Sites, Carrier Proteins, Circular Dichroism, Humans, Models, Molecular, Mutation, Nuclear Proteins, Protein Conformation, Protein Structure, Secondary, Protein Structure, Tertiary, Rats, Surface Plasmon Resonance, Polycystic kidney disease, Protein-protein interaction, Polymerization, Crystal structure

Abstract

BackgroundAutosomal dominant polycystic kidney disease (ADPKD) is the most common genetic disorder leading to end-stage renal failure in humans. In the PKD/Mhm(cy/+) rat model of ADPKD, the point mutation R823W in the sterile alpha motif (SAM) domain of the protein ANKS6 is responsible for disease. SAM domains are known protein-protein interaction domains, capable of binding each other to form polymers and heterodimers. Despite its physiological importance, little is known about the function of ANKS6 and how the R823W point mutation leads to PKD. Recent work has revealed that ANKS6 interacts with a related protein called ANKS3. Both ANKS6 and ANKS3 have a similar domain structure, with ankyrin repeats at the N-terminus and a SAM domain at the C-terminus.ResultsThe SAM domain of ANKS3 is identified as a direct binding partner of the ANKS6 SAM domain. We find that ANKS3-SAM polymerizes and ANKS6-SAM can bind to one end of the polymer. We present crystal structures of both the ANKS3-SAM polymer and the ANKS3-SAM/ANKS6-SAM complex, revealing the molecular details of their association. We also learn how the R823W mutation disrupts ANKS6 function by dramatically destabilizing the SAM domain such that the interaction with ANKS3-SAM is lost.ConclusionsANKS3 is a direct interacting partner of ANKS6. By structurally and biochemically characterizing the interaction between the ANKS3 and ANKS6 SAM domains, our work provides a basis for future investigation of how the interaction between these proteins mediates kidney function.

Published

2014

31. Orientia tsutsugamushi Nucleomodulin Ank13 Exploits the RaDAR Nuclear Import Pathway To Modulate Host Cell Transcription

Author

Haley E. Adcox, Amanda L. Hatke, Shelby E. Andersen, Sarika Gupta, Nathan B. Otto, Mary M. Weber, Richard T. Marconi, and Jason A. Carlyon

Subjects

Orientia tsutsugamushi, Rickettsia, ankyrin repeat, bacterial effector, intracellular bacterium, nucleomodulin, Microbiology, QR1-502

Abstract

ABSTRACT Orientia tsutsugamushi is the etiologic agent of scrub typhus, the deadliest of all diseases caused by obligate intracellular bacteria. Nucleomodulins, bacterial effectors that dysregulate eukaryotic transcription, are being increasingly recognized as key virulence factors. How they translocate into the nucleus and their functionally essential domains are poorly defined. We demonstrate that Ank13, an O. tsutsugamushi effector conserved among clinical isolates and expressed during infection, localizes to the nucleus in an importin β1-independent manner. Rather, Ank13 nucleotropism requires an isoleucine at the thirteenth position of its fourth ankyrin repeat, consistent with utilization of eukaryotic RaDAR (RanGDP-ankyrin repeats) nuclear import. RNA-seq analyses of cells expressing green fluorescent protein (GFP)-tagged Ank13, nucleotropism-deficient Ank13I127R, or Ank13ΔF-box, which lacks the F-box domain essential for interacting with SCF ubiquitin ligase, revealed Ank13 to be a nucleomodulin that predominantly downregulates transcription of more than 2,000 genes. Its ability to do so involves its nucleotropism and F-box in synergistic and mutually exclusive manners. Ank13 also acts in the cytoplasm to dysregulate smaller cohorts of genes. The effector’s toxicity in yeast heavily depends on its F-box and less so on its nucleotropism. Genes negatively regulated by Ank13 include those involved in the inflammatory response, transcriptional control, and epigenetics. Importantly, the majority of genes that GFP-Ank13 most strongly downregulates are quiescent or repressed in O. tsutsugamushi-infected cells when Ank13 expression is strongest. Ank13 is the first nucleomodulin identified to coopt RaDAR and a multifaceted effector that functions in the nucleus and cytoplasm via F-box-dependent and -independent mechanisms to globally reprogram host cell transcription. IMPORTANCE Nucleomodulins are recently defined effectors used by diverse intracellular bacteria to manipulate eukaryotic gene expression and convert host cells into hospitable niches. How nucleomodulins enter the nucleus, their functional domains, and the genes that they modulate are incompletely characterized. Orientia tsutsugamushi is an intracellular bacterial pathogen that causes scrub typhus, which can be fatal. O. tsutsugamushi Ank13 is the first example of a microbial protein that coopts eukaryotic RaDAR (RanGDP-ankyrin repeats) nuclear import. It dysregulates expression of a multitude of host genes with those involved in transcriptional control and the inflammatory response being among the most prominent. Ank13 does so via mechanisms that are dependent and independent of both its nucleotropism and eukaryotic-like F-box domain that interfaces with ubiquitin ligase machinery. Nearly all the genes most strongly downregulated by ectopically expressed Ank13 are repressed in O. tsutsugamushi-infected cells, implicating its importance for intracellular colonization and scrub typhus molecular pathogenesis.

Published

2021

32. Probing Muscle Ankyrin‐Repeat Protein (MARP) Structure and Function

Author

Lun, Alexander Shiang, Chen, Ju, and Lange, Stephan

Subjects

2.1 Biological and endogenous factors, 1.1 Normal biological development and functioning, Underpinning research, Aetiology, Musculoskeletal, Animals, Ankyrin Repeat, Binding Sites, COS Cells, Chlorocebus aethiops, Connectin, Cyclic AMP-Dependent Protein Kinases, Humans, Muscle Proteins, Muscle, Skeletal, Mutation, Myocardium, Nuclear Proteins, Phosphorylation, Protein Conformation, Protein Interaction Domains and Motifs, Protein Kinase C, Protein Multimerization, Protein Processing, Post-Translational, Repressor Proteins, Structure-Activity Relationship, Transfection, muscle, MARP, titin, phosphorylation, kinase, Biological Sciences, Medical and Health Sciences, Anatomy & Morphology

Abstract

Muscle ankyrin-repeat proteins (MARPs) have been shown to serve diverse functions within cardiac and skeletal muscle cells. Apart from their interactions with sarcomeric proteins like titin or myopalladin that locate them along myofilaments, MARPs are able to shuttle to the nucleus where they act as modulators for a variety of transcription factors. The deregulation of MARPs in many cardiac and skeletal myopathies contributes to their use as biomarkers for these diseases. Many of their functions are attributed to their domain composition. MARPs consist of an N-terminal coiled-coil domain responsible for their dimerization. The C-terminus contains a series of ankyrin repeats, whose best-characterized function is to bind to the N2A region of the giant sarcomeric protein titin. Here we investigate the nature of their dimerization and their interaction with titin more closely. We demonstrate that the coiled-coil domain in all MARPs enables their homo- and hetero-dimerization in antiparallel fashion. Protein complementation experiments indicate further antiparallel binding of the ankyrin repeats to titin's N2A region. Binding of MARP to titin also affects its PKA mediated phosphorylation. We demonstrate further that MARPs themselves are phosphorylated by PKA and PKC, potentially altering their structure or function. These studies elucidate structural relationships within the stretch-responsive MARP/titin complex in cross-striated muscle cells, and may relate to disease relevant posttranslational modifications of MARPs and titin that alter muscle compliance.

Published

2014

33. 辅助蛋白基因的剪接对磷脂酶A1酶活的影响.

Author

杨 蒙, 薛正莲, 甘玉飞, 周 杰, 王 洲, and 刘 艳

Subjects

REGULATOR genes, GENES, GENETIC engineering, PHOSPHOLIPASES, RESPONSE surfaces (Statistics)

Abstract

Copyright of Shipin Kexue/ Food Science is the property of Food Science Editorial Department and its content may not be copied or emailed to multiple sites or posted to a listserv without the copyright holder's express written permission. However, users may print, download, or email articles for individual use. This abstract may be abridged. No warranty is given about the accuracy of the copy. Users should refer to the original published version of the material for the full abstract. (Copyright applies to all Abstracts.)

Published

2021

34. Structure of the Legionella effector AnkX reveals the mechanism of phosphocholine transfer by the FIC domain.

Author

Campanacci, Valérie, Mukherjee, Shaeri, Roy, Craig R, and Cherfils, Jacqueline

Subjects

Legionella pneumophila, Phosphorylcholine, Bacterial Proteins, Crystallography, X-Ray, Catalytic Domain, Ankyrin Repeat, Protein Conformation, Protein Structure, Tertiary, Models, Molecular, Infectious Diseases, Infection, Biological Sciences, Information and Computing Sciences, Medical and Health Sciences, Developmental Biology

Abstract

The FIC motif and the eukaryotic-like ankyrin repeats are found in many bacterial type IV effectors, yet little is known about how these domains enable bacteria to modulate host cell functions. Bacterial FIC domains typically bind ATP and transfer adenosine monophosphate moiety onto target proteins. The ankyrin repeat-containing protein AnkX encoded by the intracellular pathogen Legionella pneumophila is unique in that its FIC domain binds to CDP-choline and transfers a phosphocholine residue onto proteins in the Rab1 GTPase family. By determining the structures of unbound AnkX and AnkX with bound CDP-choline, CMP/phosphocholine and CMP, we demonstrate that the orientation of substrate binding in relation to the catalytic FIC motif enables this protein to function as a phosphocholinating enzyme rather than a nucleotidyl transferase. Additionally, the structure reveals that the ankyrin repeats mediate scaffolding interactions that resemble those found in protein-protein interactions, but are unprecedented in intramolecular interactions. Together with phosphocholination experiments, our structures unify a general phosphoryl transferase mechanism common to all FIC enzymes that should be conserved from bacteria to human.

Published

2013

35. Honokiol targeting ankyrin repeat domain of TRPV4 ameliorates endothelial permeability in mice inflammatory bowel disease induced by DSS.

Author

Niu L, Wang S, Xu Y, Zu X, You X, Zhang Q, Zhuang P, Jiang M, Gao J, Hou X, Zhang Y, Bai G, and Deng J

Subjects

Mice, Animals, Endothelial Cells, TRPV Cation Channels metabolism, Calcium metabolism, Molecular Docking Simulation, Permeability, Ankyrin Repeat, Inflammatory Bowel Diseases drug therapy, Inflammatory Bowel Diseases metabolism, Allyl Compounds, Biphenyl Compounds, Phenols

Abstract

Ethnopharmacological Relevance: As a classic traditional Chinese medicine, Magnolia officinalis (M. officinalis) is widely used in digestive diseases. It has rich gastrointestinal activity including inflammatory bowel disease (IBD) treatment, but the mechanism is not clear., Aim of the Study: In recent years, there has been a growing interest in investigating the regulatory effects of herbal compounds on transient receptor potential (TRP) channel proteins. Transient receptor potential vanilloid 4 (TRPV4), a subtype involved in endothelial permeability regulation, was discussed as the target of M. officinalis in the treatment of IBD in the study. Based on the targeting effect of TRPV4, this study investigated the active ingredients and mechanism of M. officinalis extract in treating IBD., Materials and Methods: To reveal the connection between the active ingredients in M. officinalis and TRPV4, a bioactivity-guided high performance liquid chromatography system coupled with mass spectrometry identification was utilized to screen for TRPV4 antagonists. TRPV4 siRNA knockdown experiment was employed to validate the significance of TRPV4 as a crucial target in regulating endothelial permeability by honokiol (HON). The interaction of the active ingredient representing HON with TRPV4 was confirmed by molecular docking, fluorescence-based thermal shift and live cell calcium imaging experiments. The potential binding sites and inhibitory mechanisms of HON in TRPV4 were analyzed by molecular dynamics simulation and microscale thermophoresis. The therapeutic effect of HON based on TRPV4 was discussed in DSS-IBD mice., Results: Our finding elucidated that the inhibitory activity of M. officinalis against TRPV4 is primarily attributed to HON analogues. The knockdown of TRPV4 expression significantly impaired the calcium regulation and permeability protection in endothelial cells. The mechanism study revealed that HON specifically targets the Q239 residue located in the ankyrin repeat domain of TRPV4, and competitively inhibits channel opening with adenosine triphosphate (ATP) binding. The immunofluorescence assay demonstrated that the administration of HON enhances the expression and location of VE-Cadherin to protect the endothelial barrier and attenuates immune cell infiltration., Conclusions: The finding suggested that HON alleviates IBD by improving endothelial permeability through TRPV4. The discovery provides valuable insights into the potential therapeutic strategy of active natural products for alleviating IBD., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier B.V. All rights reserved.)

Published

2024

36. Preclinical Evaluation of HER2-Targeting DARPin G3: Impact of Albumin-Binding Domain (ABD) Fusion.

Author

Deyev SM, Oroujeni M, Garousi J, Gräslund T, Li R, Rosly AHB, Orlova A, Konovalova E, Schulga A, Vorobyeva A, and Tolmachev V

Subjects

Animals, Female, Humans, Mice, Albumins metabolism, Ankyrin Repeat, Cell Line, Tumor, Lutetium, Protein Binding, Protein Domains, Radioisotopes, Radiopharmaceuticals metabolism, Recombinant Fusion Proteins metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins chemistry, Tissue Distribution, Molecular Targeted Therapy, Receptor, ErbB-2 antagonists & inhibitors

Abstract

Designed ankyrin repeat protein (DARPin) G3 is an engineered scaffold protein. This small (14.5 kDa) targeting protein binds with high affinity to human epidermal growth factor receptor 2 (HER2). HER2 is overexpressed in several cancers. The use of the DARPin G3 for radionuclide therapy is complicated by its high renal reabsorption after clearance via the glomeruli. We tested the hypothesis that a fusion of the DARPin G3 with an albumin-binding domain (ABD) would prevent rapid renal excretion and high renal reabsorption resulting in better tumour targeting. Two fusion proteins were produced, one with the ABD at the C-terminus (G3-ABD) and another at the N-terminus (ABD-G3). Both variants were labelled with 177 Lu. The binding properties of the novel constructs were evaluated in vitro and their biodistribution was compared in mice with implanted human HER2-expressing tumours. Fusion with the ABD increased the retention time of both constructs in blood compared with the non-ABD-fused control. The effect of fusion with the ABD depended strongly on the order of the domains in the constructs, resulting in appreciably better targeting properties of [ 177 Lu]Lu-G3-ABD. Our data suggest that the order of domains is critical for the design of targeting constructs based on scaffold proteins.

Published

2024

37. Identification of ANKDD1B variants in an ankylosing spondylitis pedigree and a sporadic patient

Author

Zhiping Tan, Hui Zeng, Zhaofa Xu, Qi Tian, Xiaoyang Gao, Chuanman Zhou, Yu Zheng, Jian Wang, Guanghui Ling, Bing Wang, Yifeng Yang, and Long Ma

Subjects

Ankylosing spondylitis, Pedigree, ANKDD1B, Ankyrin repeat, HLA-B*27, Internal medicine, RC31-1245, Genetics, QH426-470

Abstract

Abstract Background Ankylosing spondylitis (AS) is a debilitating autoimmune disease affecting tens of millions of people in the world. The genetics of AS is unclear. Analysis of rare AS pedigrees might facilitate our understanding of AS pathogenesis. Methods We used genome-wide linkage analysis and whole-exome sequencing in combination with variant co-segregation verification and haplotype analysis to study an AS pedigree and a sporadic AS patient. Results We identified a missense variant in the ankyrin repeat and death domain containing 1B gene ANKDD1B from a Han Chinese pedigree with dominantly inherited AS. This variant (p.L87V) co-segregates with all male patients of the pedigree. In females, the penetrance of the symptoms is incomplete with one identified patient out of 5 carriers, consistent with the reduced frequency of AS in females of the general population. We further identified a distinct missense variant affecting a conserved amino acid (p.R102L) of ANKDD1B in a male from 30 sporadic early onset AS patients. Both variants are absent in 500 normal controls. We determined the haplotypes of four major known AS risk loci, including HLA-B*27, 2p15, ERAP1 and IL23R, and found that only HLA-B*27 is strongly associated with patients in our cohort. Conclusions Together these results suggest that ANKDD1B variants might be associated with AS and genetic analyses of more AS patients are warranted to verify this association.

Published

2018

38. Chaperone function of Arabidopsis NPR1.

Author

Paeng, Seol Ki, Chi, Yong Hun, Kang, Chang Ho, Chae, Ho Byoung, Lee, Eun Seon, Park, Joung Hun, Wi, Seong Dong, Bae, Su Bin, Phan, Kieu Anh Thi, and Lee, Sang Yeol

Subjects

*SESSILE organisms, *MOLECULAR structure, *ARABIDOPSIS, *PROTEIN-protein interactions, *MOLECULAR chaperones, *HEAT shock proteins, *MONOMERS

Abstract

To cope with diverse environmental stresses, the sessile organisms of plants have evolved diverse defense molecules and signaling systems to transfer the stress signals into downstream metabolic cascades and induce the expression of defense-associated genes. Among the defense systems, the Arabidopsis nonexpressor of pathogenesis-related protein 1 (AtNPR1) playing a key role in a plant systemic acquired immune responses has been shown to have multiple functions. The molecular structure of AtNPR1 has two domains, BTB/POZ and ANK repeat, that are involved in protein–protein interactions. Despite the function of its salicylic acid-induced defense activity in nucleus, the biochemical property of its cytosolic oligomers has not been elucidated. Based on the results that the reversible structural change of redox proteins is a typical property of molecular chaperones, we investigated the biochemical characteristics of AtNPR1 after expressing it in E. coli and purifying the protein. From the study, the recombinant AtNPR1 functions as a protein chaperone to protect plants from heat stress through its structural switching by its oligomer form. Under heat-induced (43 °C) condition, the AtNPR1 protein prevents from aggregation of substrate, MDH. And the structural change was regulated upon the redox changes, such as DTT treatment dissociated its structure to monomer and reduced its chaperone activity, suggesting that the heat-induced chaperone activity of AtNPR1 is dependent on its redox status. In summary, the cytosolic AtNPR1 oligomer performs the important function of molecular chaperone to protect plants from heat stress that can be applied to the preparation of heat shock-tolerant useful crops. [ABSTRACT FROM AUTHOR]

Published

2020

39. Functional Dynamics of the Folded Ankyrin Repeats of IκBα Revealed by Nuclear Magnetic Resonance

Author

Cervantes, Carla F, Markwick, Phineus RL, Sue, Shih-Che, McCammon, J Andrew, Dyson, H Jane, and Komives, Elizabeth A

Subjects

Biochemistry and Cell Biology, Biological Sciences, Amino Acid Sequence, Animals, Ankyrin Repeat, Deuterium Exchange Measurement, Humans, I-kappa B Kinase, Mice, Molecular Sequence Data, Nuclear Magnetic Resonance, Biomolecular, Peptide Fragments, Protein Binding, Protein Folding, Protein Structure, Secondary, Protein Structure, Tertiary, Sequence Alignment, Thermodynamics, Medicinal and Biomolecular Chemistry, Medical Biochemistry and Metabolomics, Biochemistry & Molecular Biology, Biochemistry and cell biology, Medical biochemistry and metabolomics, Medicinal and biomolecular chemistry

Abstract

Inhibition of nuclear factor kappaB (NF-kappaB) is mainly accomplished by IkappaB alpha, which consists of a signal response sequence at the N-terminus, a six-ankyrin repeat domain (ARD) that binds NF-kappaB, and a C-terminal PEST sequence. Previous studies with the ARD revealed that the fifth and sixth repeats are only partially folded in the absence of NF-kappaB. Here we report NMR studies of a truncated version of IkappaB alpha, containing only the first four ankyrin repeats, IkappaB alpha(67-206). This four-repeat segment is well-structured in the free state, enabling full resonance assignments to be made. H-D exchange, backbone dynamics, and residual dipolar coupling (RDC) experiments reveal regions of flexibility. In addition, regions consistent with the presence of micro- to millisecond motions occur periodically throughout the repeat structure. Comparison of the RDCs with the crystal structure gave only moderate agreement, but an ensemble of structures generated by accelerated molecular dynamics gave much better agreement with the measured RDCs. The regions showing flexibility correspond to those implicated in entropic compensation for the loss of flexibility in ankyrin repeats 5 and 6 upon binding to NF-kappaB. The regions showing micro- to millisecond motions in the free protein are the ends of the beta-hairpins that directly interact with NF-kappaB in the complex.

Published

2009

40. Functional dynamics of the folded ankyrin repeats of I kappa B alpha revealed by nuclear magnetic resonance.

Author

Cervantes, Carla F, Markwick, Phineus RL, Sue, Shih-Che, McCammon, J Andrew, Dyson, H Jane, and Komives, Elizabeth A

Subjects

Animals, Humans, Mice, Peptide Fragments, Deuterium Exchange Measurement, Nuclear Magnetic Resonance, Biomolecular, Sequence Alignment, Amino Acid Sequence, Ankyrin Repeat, Protein Structure, Secondary, Protein Structure, Tertiary, Protein Binding, Protein Folding, Thermodynamics, Molecular Sequence Data, I-kappa B Kinase, Nuclear Magnetic Resonance, Biomolecular, Protein Structure, Secondary, Tertiary, Medicinal and Biomolecular Chemistry, Biochemistry and Cell Biology, Medical Biochemistry and Metabolomics, Biochemistry & Molecular Biology

Abstract

Inhibition of nuclear factor kappaB (NF-kappaB) is mainly accomplished by IkappaB alpha, which consists of a signal response sequence at the N-terminus, a six-ankyrin repeat domain (ARD) that binds NF-kappaB, and a C-terminal PEST sequence. Previous studies with the ARD revealed that the fifth and sixth repeats are only partially folded in the absence of NF-kappaB. Here we report NMR studies of a truncated version of IkappaB alpha, containing only the first four ankyrin repeats, IkappaB alpha(67-206). This four-repeat segment is well-structured in the free state, enabling full resonance assignments to be made. H-D exchange, backbone dynamics, and residual dipolar coupling (RDC) experiments reveal regions of flexibility. In addition, regions consistent with the presence of micro- to millisecond motions occur periodically throughout the repeat structure. Comparison of the RDCs with the crystal structure gave only moderate agreement, but an ensemble of structures generated by accelerated molecular dynamics gave much better agreement with the measured RDCs. The regions showing flexibility correspond to those implicated in entropic compensation for the loss of flexibility in ankyrin repeats 5 and 6 upon binding to NF-kappaB. The regions showing micro- to millisecond motions in the free protein are the ends of the beta-hairpins that directly interact with NF-kappaB in the complex.

Published

2009

41. Microbial Enzymes for Conversion of Biomass to Bioenergy

Author

Raghavendra, M. P., Nayaka, S. Chandra, Gupta, Vijai Kumar, Gupta, Vijai Kumar, Series editor, and Tuohy, Maria G., Series editor

Published

2016

42. Epidemiology, Molecular Biology, and Pathogenic Mechanisms of Ehrlichia Infections

Author

Yu, Xue-jie, Walker, David H., and Thomas, Sunil, editor

Published

2016

43. Methyl-Lysine Recognition by Ankyrin-Repeat Proteins

Author

Collins, Robert E., Cheng, Xiaodong, and Zhou, Ming-Ming, editor

Published

2015

44. Biorecognition Molecules: Types and Molecular Basis and Development of Specificity

Author

Collins, Robert E., Cortajarena, Aitziber L., Rodríguez-Hernández, Juan, editor, and Cortajarena, Aitziber L., editor

Published

2015

45. Coordinated methyl readers: Functional communications in cancer

Author

Ji Min Lee, Minsol Jeon, Il Geun Park, and Hyun-Kyung Kim

Subjects

0301 basic medicine, Cancer Research, Methyltransferase, biology, Chemistry, Lysine, Methyltransferases, Methylation, Chromodomain, Cell biology, Histones, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, Histone, Non-histone protein, Neoplasms, 030220 oncology & carcinogenesis, biology.protein, Humans, Ankyrin repeat, Epigenetics, Target protein

Abstract

Methylation is a major post-translational modification (PTM) generated by methyltransferase on target proteins; it is recognized by the epigenetic reader to expand the functional diversity of proteins. Methylation can occur on specific lysine or arginine residues localized within regulatory domains in both histone and nonhistone proteins, thereby allowing distinguished properties of the targeted protein. Methylated residues are recognized by chromodomain, malignant brain tumor (MBT), Tudor, plant homeodomain (PHD), PWWP, WD-40, ADD, and ankyrin repeats by an induced-fit mechanism. Methylation-dependent activities regulate distinct aspects of target protein function and are largely reliant on methyl readers of histone and nonhistone proteins in various diseases. Methylation of nonhistone proteins that are recognized by methyl readers facilitates the degradation of unwanted proteins, as well as the stabilization of necessary proteins. Unlike nonhistone substrates, which are mainly monomethylated by methyltransferase, histones are di- or trimethylated by the same methyltransferases and then connected to other critical regulators by methyl readers. These fine-tuned controls by methyl readers are significant for the progression or inhibition of diseases, including cancers. Here, current knowledge and our perspectives about regulating protein function by methyl readers are summarized. We also propose that expanded research on the strong crosstalk mechanisms between methylation and other PTMs via methyl readers would augment therapeutic research in cancer.

Published

2022

46. Interactome of the Autoimmune Risk Protein ANKRD55

Author

Nerea Ugidos, Jorge Mena, Sara Baquero, Iraide Alloza, Mikel Azkargorta, Felix Elortza, and Koen Vandenbroeck

Subjects

ANKRD55, ankyrin repeat, autoimmune, multiple sclerosis, rheumatoid arthritis, Immunologic diseases. Allergy, RC581-607

Abstract

The ankyrin repeat domain-55 (ANKRD55) gene contains intronic single nucleotide polymorphisms (SNPs) associated with risk to contract multiple sclerosis, rheumatoid arthritis or other autoimmune disorders. Risk alleles of these SNPs are associated with higher levels of ANKRD55 in CD4+ T cells. The biological function of ANKRD55 is unknown, but given that ankyrin repeat domains constitute one of the most common protein-protein interaction platforms in nature, it is likely to function in complex with other proteins. Thus, identification of its protein interactomes may provide clues. We identified ANKRD55 interactomes via recombinant overexpression in HEK293 or HeLa cells and mass spectrometry. One hundred forty-eight specifically interacting proteins were found in total protein extracts and 22 in extracts of sucrose gradient-purified nuclei. Bioinformatic analysis suggested that the ANKRD55-protein partners from total protein extracts were related to nucleotide and ATP binding, enriched in nuclear transport terms and associated with cell cycle and RNA, lipid and amino acid metabolism. The enrichment analysis of the ANKRD55-protein partners from nuclear extracts is related to sumoylation, RNA binding, processes associated with cell cycle, RNA transport, nucleotide and ATP binding. The interaction between overexpressed ANKRD55 isoform 001 and endogenous RPS3, the cohesins SMC1A and SMC3, CLTC, PRKDC, VIM, β-tubulin isoforms, and 14-3-3 isoforms were validated by western blot, reverse immunoprecipitaton and/or confocal microscopy. We also identified three phosphorylation sites in ANKRD55, with S436 exhibiting the highest score as likely 14-3-3 binding phosphosite. Our study suggests that ANKRD55 may exert function(s) in the formation or architecture of multiple protein complexes, and is regulated by (de)phosphorylation reactions. Based on interactome and subcellular localization analysis, ANKRD55 is likely transported into the nucleus by the classical nuclear import pathway and is involved in mitosis, probably via effects associated with mitotic spindle dynamics.

Published

2019

47. Whole-Genome Comparisons Among the Genus Shewanella Reveal the Enrichment of Genes Encoding Ankyrin-Repeats Containing Proteins in Sponge-Associated Bacteria

Author

Anoop Alex and Agostinho Antunes

Subjects

sponge-microbe symbiosis, Shewanella, adaptation, eukaryotic-like proteins, ankyrin repeat, Microbiology, QR1-502

Abstract

The bacterial members of the genus Shewanella are widely distributed and inhabit both freshwater and marine environments. Some members of Shewanella have gained considerable attention due to its ability to survive in redox-stratified environments. However, a gap of knowledge exists on the key genomic features of the sponge-associated Shewanella sp. involving the successful host-bacteria interaction, as sponge-symbiotic Shewanella are largely underrepresented in the public repositories. With the aim of identifying the genomic signatures of sponge-Shewanella association, we generated a high-quality genome data of a sponge-associated, Shewanella sp. OPT22, isolated from the intertidal marine sponge Ophlitaspongia papilla and performed comprehensive comparative analyses of 68 genome strains of the genus Shewanella including two previously reported genomes of sponge-associated bacteria, Shewanella spongiae KCTC 22492 and Shewanella sp. Alg231_23. The 16S rRNA-based phylogenetic reconstruction showed the well-supported affiliation of OPT22 and KCTC 22492 with previously reported sponge-associated bacteria, affirming the “sponge-specific” nature of these two bacterial strains isolated from different marine sponge species from the Atlantic and Pacific (East Sea) Oceans, respectively. The genome comparison of the 68 strains of Shewanella inhabiting different habitats revealed the unusual/previously unreported abundance of genes encoding for ankyrin-repeat containing proteins (ANKs) in the genomes of the two sponge-associated strains, OPT22 (ANKs; n = 45) and KCTC 22492 (ANKs; n = 52), which might be involved in sponge-Shewanella interactions. Focused analyses detected the syntenic organization of the gene cluster encoding major secretion system (type III/IV/VI) components and the presence of effector homologs in OPT22 and KCTC 22492 that seem to play a role in the virulence of the sponge bacteria. The genomic island (GI) of Shewanella sp. OPT22 was identified to localize a gene cluster encoding T4SS components and ANK (n = 1), whereas S. spongiae KCTC 22492 harbored a total of seven ANKs within multiple GIs. GIs may play a pivotal role in the dissemination of symbioses-related genes (ANKs) through the horizontal gene transfer, contributing to the diversification and adaptation of sponge-associated Shewanella. Overall, the genome analyses of Shewanella isolates from marine sponges revealed genomic repertoires that might be involved in establishing successful symbiotic relationships with the sponge hosts.

Published

2019

48. Deciphering the roles of subcellular distribution and interactions involving the MEF2 binding region, the ankyrin repeat binding motif and the catalytic site of HDAC4 in Drosophila neuronal morphogenesis.

Author

Tan WJ, Hawley HR, Wilson SJ, and Fitzsimons HL

Subjects

Animals, Catalytic Domain, Cell Nucleus metabolism, MEF2 Transcription Factors genetics, MEF2 Transcription Factors metabolism, Morphogenesis, Neurons metabolism, Ankyrin Repeat, Drosophila metabolism, Histone Deacetylases genetics, Histone Deacetylases metabolism

Abstract

Background: Dysregulation of nucleocytoplasmic shuttling of histone deacetylase 4 (HDAC4) is associated with several neurodevelopmental and neurodegenerative disorders. Consequently, understanding the roles of nuclear and cytoplasmic HDAC4 along with the mechanisms that regulate nuclear entry and exit is an area of concerted effort. Efficient nuclear entry is dependent on binding of the transcription factor MEF2, as mutations in the MEF2 binding region result in cytoplasmic accumulation of HDAC4. It is well established that nuclear exit and cytoplasmic retention are dependent on 14-3-3-binding, and mutations that affect binding are widely used to induce nuclear accumulation of HDAC4. While regulation of HDAC4 shuttling is clearly important, there is a gap in understanding of how the nuclear and cytoplasmic distribution of HDAC4 impacts its function. Furthermore, it is unclear whether other features of the protein including the catalytic site, the MEF2-binding region and/or the ankyrin repeat binding motif influence the distribution and/or activity of HDAC4 in neurons. Since HDAC4 functions are conserved in Drosophila, and increased nuclear accumulation of HDAC4 also results in impaired neurodevelopment, we used Drosophila as a genetic model for investigation of HDAC4 function., Results: Here we have generated a series of mutants for functional dissection of HDAC4 via in-depth examination of the resulting subcellular distribution and nuclear aggregation, and correlate these with developmental phenotypes resulting from their expression in well-established models of neuronal morphogenesis of the Drosophila mushroom body and eye. We found that in the mushroom body, forced sequestration of HDAC4 in the nucleus or the cytoplasm resulted in defects in axon morphogenesis. The actions of HDAC4 that resulted in impaired development were dependent on the MEF2 binding region, modulated by the ankyrin repeat binding motif, and largely independent of an intact catalytic site. In contrast, disruption to eye development was largely independent of MEF2 binding but mutation of the catalytic site significantly reduced the phenotype, indicating that HDAC4 acts in a neuronal-subtype-specific manner., Conclusions: We found that the impairments to mushroom body and eye development resulting from nuclear accumulation of HDAC4 were exacerbated by mutation of the ankyrin repeat binding motif, whereas there was a differing requirement for the MEF2 binding site and an intact catalytic site. It will be of importance to determine the binding partners of HDAC4 in nuclear aggregates and in the cytoplasm of these tissues to further understand its mechanisms of action., (© 2023. The Author(s).)

Published

2024

49. Structural Biology of TRP Channels

Author

Hellmich, Ute A., Gaudet, Rachelle, Rosenthal, W., Series editor, Barrett, James E., Series editor, Buckingham, Julia, Series editor, Flockerzi, Veit, Series editor, Geppetti, Pierangelo, Series editor, Hofmann, Franz B., Series editor, Michel, Martin C., Series editor, Moore, Philip, Series editor, Page, Clive P., Series editor, and Nilius, Bernd, editor

Published

2014

50. Interactome of the Autoimmune Risk Protein ANKRD55.

Author

Ugidos, Nerea, Mena, Jorge, Baquero, Sara, Alloza, Iraide, Azkargorta, Mikel, Elortza, Felix, and Vandenbroeck, Koen

Subjects

PROTEOMICS, SINGLE nucleotide polymorphisms, AMINO acid metabolism, SPINDLE apparatus, PROTEINS, PROTEIN-protein interactions, AUTOIMMUNE diseases

Abstract

The ankyrin repeat domain-55 (ANKRD55) gene contains intronic single nucleotide polymorphisms (SNPs) associated with risk to contract multiple sclerosis, rheumatoid arthritis or other autoimmune disorders. Risk alleles of these SNPs are associated with higher levels of ANKRD55 in CD4+ T cells. The biological function of ANKRD55 is unknown, but given that ankyrin repeat domains constitute one of the most common protein-protein interaction platforms in nature, it is likely to function in complex with other proteins. Thus, identification of its protein interactomes may provide clues. We identified ANKRD55 interactomes via recombinant overexpression in HEK293 or HeLa cells and mass spectrometry. One hundred forty-eight specifically interacting proteins were found in total protein extracts and 22 in extracts of sucrose gradient-purified nuclei. Bioinformatic analysis suggested that the ANKRD55-protein partners from total protein extracts were related to nucleotide and ATP binding, enriched in nuclear transport terms and associated with cell cycle and RNA, lipid and amino acid metabolism. The enrichment analysis of the ANKRD55-protein partners from nuclear extracts is related to sumoylation, RNA binding, processes associated with cell cycle, RNA transport, nucleotide and ATP binding. The interaction between overexpressed ANKRD55 isoform 001 and endogenous RPS3, the cohesins SMC1A and SMC3, CLTC, PRKDC, VIM, β-tubulin isoforms, and 14-3-3 isoforms were validated by western blot, reverse immunoprecipitaton and/or confocal microscopy. We also identified three phosphorylation sites in ANKRD55, with S436 exhibiting the highest score as likely 14-3-3 binding phosphosite. Our study suggests that ANKRD55 may exert function(s) in the formation or architecture of multiple protein complexes, and is regulated by (de)phosphorylation reactions. Based on interactome and subcellular localization analysis, ANKRD55 is likely transported into the nucleus by the classical nuclear import pathway and is involved in mitosis, probably via effects associated with mitotic spindle dynamics. [ABSTRACT FROM AUTHOR]

Published

2019