Your search keyword '"Electroelution"' showing total 531 results

1. Identification and Activity Study of an Impurity Band Observed in the nrSDS-PAGE of Aflibercept

Author

Li, Meng, Li, Weiyu, Wang, Xin, Wu, Gang, Du, Jialiang, Xu, Gangling, Duan, Maoqin, Yu, Xiaojuan, Cui, Chunbo, Liu, Chunyu, Fu, Zhihao, Yu, Chuanfei, and Wang, Lan

Published

2024

2. Electroelution of 31 kDa Immunogenic Protein Fraction from the Salivary Gland of Aedes aegypti and Aedes albopictus (Diptera: Culicidae)

Author

Zakiyyah, Ilma, Santika, Linda Dwi, Wathon, Syubbanul, Senjarini, Kartika, Oktarianti, Rike, Ma, Wanshu, Series Editor, Lelono, Asmoro, editor, Akbar Bahar, Muhammad, editor, Wathon, Syubanul, editor, Senjarini, Kartika, editor, Ginanjar Arip, Asep, editor, Putrasetya, Ramdhan, editor, Andika, Beny, editor, Ayu Sukma, Nadhea, editor, and Sugiharto, Bambang, Editor-in-Chief

Published

2023

3. Gel Protein Extraction's Impact on Conformational Epitopes of Linear Non-Tagged MPT64 Protein.

Author

Kusuma, Sri Agung Fitri, Fadhlillah, Muhammad, Rostinawati, Tina, Maisyarah, Intan Timur, Syafitri, Raden Indah Puspita, and Subroto, Toto

Subjects

RECOMBINANT proteins, EPITOPES, ELECTROPHORESIS, WESTERN immunoblotting, IMMUNOGLOBULIN G

Abstract

The production and purification of recombinant proteins are crucial to acquiring pure MPT64 protein. Due to the fact that protein epitopes may undergo conformational changes during purification, this study, therefore, investigated an effective rapid purification method to produce highly intracellular pure MPT64 protein without causing conformational changes in the epitope under denaturing conditions. MPT64 was isolated from E. coli and electrophoresed using gel SDS-PAGE. Then, the desired protein bands were excised and purified with two methods: electroelution and passive elution. The isolated protein was identified via peptide mass fingerprinting using MALDI-TOF MS and reacted with IgG anti-MPT64, and the cross-reactivity of the isolated protein with IgY anti-MPT64 was confirmed using Western blot. The results show that both of these methods produced pure MPT64 protein, and the MPT64 protein was confirmed based on the MALDI-TOF MS results. Neither of these two methods resulted in epitope changes in the MPT64 protein so it could react specifically with both antibodies. The yield of MPT64 protein was higher with electroelution (2030 ± 41 µg/mL) than with passive elution (179.5 ± 7.5 µg/mL). Thus, it can be inferred that the electroelution method is a more effective method of purifying MPT64 protein and maintaining its epitope than the passive elution method. [ABSTRACT FROM AUTHOR]

Published

2023

4. 牛血抗菌肽的制备及应用.

Author

王亚贝, 刘亚彬, 丁兰卉, 邓昊仁, 承佳佳, and 杨萍

Subjects

ANTIMICROBIAL peptides, POLYACRYLAMIDE gel electrophoresis, MOLECULAR weights, EXTRACTION (Chemistry), PEPTIDES, RAW materials, ULTRASONICS, CENTRIFUGATION

Abstract

Copyright of Food Research & Development is the property of Food Research & Development 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

2023

5. Gel Protein Extraction’s Impact on Conformational Epitopes of Linear Non-Tagged MPT64 Protein

Author

Sri Agung Fitri Kusuma, Muhammad Fadhlillah, Tina Rostinawati, Intan Timur Maisyarah, Raden Indah Puspita Syafitri, and Toto Subroto

Subjects

MPT64, passive elution, electroelution, non-tagged, intracellular, Science, Chemistry, QD1-999, Inorganic chemistry, QD146-197, General. Including alchemy, QD1-65

Abstract

The production and purification of recombinant proteins are crucial to acquiring pure MPT64 protein. Due to the fact that protein epitopes may undergo conformational changes during purification, this study, therefore, investigated an effective rapid purification method to produce highly intracellular pure MPT64 protein without causing conformational changes in the epitope under denaturing conditions. MPT64 was isolated from E. coli and electrophoresed using gel SDS-PAGE. Then, the desired protein bands were excised and purified with two methods: electroelution and passive elution. The isolated protein was identified via peptide mass fingerprinting using MALDI-TOF MS and reacted with IgG anti-MPT64, and the cross-reactivity of the isolated protein with IgY anti-MPT64 was confirmed using Western blot. The results show that both of these methods produced pure MPT64 protein, and the MPT64 protein was confirmed based on the MALDI-TOF MS results. Neither of these two methods resulted in epitope changes in the MPT64 protein so it could react specifically with both antibodies. The yield of MPT64 protein was higher with electroelution (2030 ± 41 µg/mL) than with passive elution (179.5 ± 7.5 µg/mL). Thus, it can be inferred that the electroelution method is a more effective method of purifying MPT64 protein and maintaining its epitope than the passive elution method.

Published

2023

6. Gel electrophoresis/electroelution sorting fractionator combined with filter‐aided sample preparation for deep proteomic analysis.

Author

Ramos, Yassel, Almeida, Alexis, Carpio, Jenis, Rodríguez‐Ulloa, Arielis, Perera, Yasser, González, Luis J., Wiśniewski, Jacek R., and Besada, Vladimir

Subjects

*POLYACRYLAMIDE gel electrophoresis, *GEL electrophoresis, *PROTEIN fractionation, *SODIUM dodecyl sulfate, *PROTEOMICS, *PEPTIDES

Abstract

Sample preparation and protein fractionation are important issues for proteomic studies. Protein extraction procedures strongly affect the performance of fractionation methods by provoking protein dispersion in several fractions. The most notable exception is the gel‐based electrophoretic protein fractionation due to its resolution and effectiveness of sodium dodecyl sulfate as a solubilizing agent, while its main limitation lies in the poor recovery of the gel‐trapped proteins. We created a fractionator device to separate complex mixture of proteins and peptides that is based on the continuous gel electrophoresis/electroelution sorting of these molecules. In an unsupervised process, complex mixtures of proteins or peptides are fractionated into the gel while separated fractions are simultaneously and sequentially electroeluted to the solution containing wells. The performance of the device was studied for protein fractionation in terms of reproducibility, protein recovery, and loading capacity. In a setup free of sodium dodecyl sulfate, complex peptide mixtures can also be fractionated. More than 11,700 proteins were identified in the whole‐cell lysate of the CaSki cell line by using the fractionator combined with the filter‐aided sample preparation method and mass spectrometry analysis. Fractionator‐based proteome characterization increased 1.7‐fold the number of identified proteins compared to the unfractionated sample analysis. [ABSTRACT FROM AUTHOR]

Published

2022

7. Experimental setup for the identification of mitochondrial protease substrates by shotgun and top-down proteomics

Author

Alice Di Pierro, Heather Bondi, Chiara Monti, Luisa Pieroni, Enrico Cilio, Andrea Urbani, Tiziana Alberio, Mauro Fasano, and Maurizio Ronci

Subjects

Mitochondria, Protease, Shotgun, Top-down, Electroelution, Genetics, QH426-470

Abstract

Mitochondria possess a proteolytic system that contributes to the regulation of mitochondrial dynamics, mitochondrial biogenesis and mitophagy. We aimed at the identification by bottom-up proteomics of altered protein processing due to the activation of mitochondrial proteases in a cellular model of impaired dopamine homeostasis. Moreover, we optimized the conditions for top-down proteomics to identify the cleavage site sequences.

Published

2016

8. A simple electroelution method for rapid protein purification: isolation and antibody production of alpha toxin from Clostridium septicum

Author

Lorena Vázquez-Iglesias, Borja Estefanell-Ucha, Leticia Barcia-Castro, María Páez de la Cadena, Paula Álvarez-Chaver, Daniel Ayude-Vázquez, and Francisco Javier Rodríguez-Berrocal

Subjects

Antibodies, Slot blot, Alpha-toxin, Electroelution, Clostridium septicum, Medicine, Biology (General), QH301-705.5

Abstract

Clostridium septicum produces a number of diseases in human and farm animals which, in most of the cases, are fatal without clinical intervention. Alpha toxin is an important agent and the unique lethal virulent factor produced by Clostridium septicum. This toxin is haemolytic, highly lethal and necrotizing activities but is being used as an antigen to develop animal vaccines. The aim of this study was to isolate the alpha toxin of Clostridium septicum and produce highly specific antibodies against it. In this work, we have developed a simple and efficient method for alpha toxin purification, based on electroelution that can be used as a time-saving method for purifying proteins. This technique avoids contamination by other proteins that could appear during other protein purification techniques such chromatography. The highly purified toxin was used to produce polyclonal antibodies. The specificity of the antibodies was tested by western blot and these antibodies can be applied to the quantitative determination of alpha toxin by slot blot.

Published

2017

9. Quantitation during Electroblotting Step : Enhanced Protein Recovery after Electrotransfer using Square Wave Alternating Voltage

Author

Bienvenut, WV., Deon, C., Sanchez, J-C., Hochstrasser, DF., and Bienvenut, Willy Vincent, editor

Published

2005

10. Comparison of simple and rapid extracting methods of free-tags Mycobacterium tuberculosis protein 64 Recombinant Protein from polyacrylamide gel: Electroelution and the optimized passive elution

Author

Asep Rizaludin, Yaya Rukayadi, Sri Agung Fitri Kusuma, Muhammad Fadhlillah, Ida Parwati, and Toto Subroto

Subjects

Gel electrophoresis, Chromatography, biology, Elution, mpt64, Sodium, chemistry.chemical_element, RM1-950, biology.organism_classification, sodium dodecyl sulfate-polyacrylamide gel electrophoresis, law.invention, Mycobacterium tuberculosis, RS1-441, Pharmacy and materia medica, chemistry, Affinity chromatography, law, Electroelution, passive elution, Recombinant DNA, Therapeutics. Pharmacology, Polyacrylamide gel electrophoresis

Abstract

In this study, the Mycobacterium tuberculosis protein 64 (MPT64) protein was constructed without any tags to facilitate the purification using column affinity chromatography, but the MPT64 must be obtained as a pure protein. This study was purpose to ensure the efficient extracting method to purify protein MPT64 directly from the polyacrylamide gel. The crude extract of extracellular protein containing MPT64 protein was separated into single protein band and the targeted protein which is located in the size of 24 kDa was excised. Each of the six bands was collected in a sterile microtube to be eluted using electroelution and the optimized of the passive-elution method. Both the elution methods demonstrated the purity level of the MPT64 protein by detecting a solely band on the gel at the 24 kDa. Among the variety of passive-elution time, the highest MPT64 protein concentration was 0.549 mg/ml after elution for 72 h. However, the electroelution result provided higher MPT64 protein concentration, i.e., 0.683 mg/mL. However, based on the recognition of the purified MPT64 protein on commercial detection kit of MPT64 protein, it showed that the positive result was only showed by the passive-elution extracting protein. Therefore, for purifying the protein MPT64 from the sodium dodecyl sulfate-polyacrylamide gel electrophoresis gels, the efficient method was passive elution.

Published

2021

11. An innovative ring-shaped electroeluter for high concentration preparative isolation of protein from polyacrylamide gel.

Author

Chen, Jing-Jing, Li, Guo-Qing, Pratush, Amit, Jahan, Sharmin, Kong, Fan-Zhi, Xiao, Hua, Fan, Liu-Yin, and Cao, Cheng-Xi

Subjects

*PROTEIN analysis, *POLYACRYLAMIDE gel electrophoresis, *ELUTION (Chromatography), *BIOMOLECULES, *BIOCHEMISTRY

Abstract

A ring-shaped electroeluter (RSE) was designed for protein recovery from polyacrylamide gel matrix. The RSE was designed in such a way that a ring-shaped well was used to place gel slices and an enrichment well was used to collect eluted protein samples. With HSA as model protein, the electroelution time was less than 30 min with 80% recovery rate, and the concentration of recovered protein was 50 times higher than that of conventional method. The RSE could be reused at least ten times. The developed device makes great advance towards economic electroelution of biomolecules (such as proteins) from gel matrix. [ABSTRACT FROM AUTHOR]

Published

2017

12. Antibacterial Activity of Isolated Immunodominant Proteins of Naja Naja (Oxiana) Venom.

Author

mehrdar, Mahboobeh talebi, hajihosseini, Reza, madani, Rasool, and bidhendid, Soheila moradi

Subjects

*ANTIBACTERIAL agents, *ANTIVENINS, *METHICILLIN-resistant staphylococcus aureus, *ESCHERICHIA coli, *BACILLUS (Bacteria), *PSEUDOMONAS

Abstract

The aim of this study is to investigate antibacterial effects of immunodominant proteins isolated from the venom of Naja Naja Oxiana snake against Staphylococcus aureus, Escherichia coli, Bacillus subtilis and Pseudomonas aeruginosa. The innate immune system is an important line of defense against bacterial diseases. Antibacterial peptides and proteins produced by snake venoms have recently attracted significant attention due to their relevance to bacterial diseases and the potential of being converted into new therapeutic agents. Identification of immunodominant proteins of the venom of Naja Naja Oxiana snake was performed by SDS-PAGE and western blot analysis. Identified proteins were isolated directly from preparative gel electrophoresis by Electro-elution. In the next step, antibacterial effects of immunodominant proteins were tested against several strains of clinical isolates, including S.aureus, B.subtilis (Gram-positive bacteria) P.aeruginosa and E.coli (Gram-negative bacteria) using broth microdilution and disc-diffusion assays. In order to compare the results of the discdiffusion assay, antibacterial effects of several antibiotics (Gentamicin, Ampicillin, Penicillin, Amoxicillin and Ciprofloxacin) were also examined using the same conditions. Results showed that immunodominant proteins of (14, and 65kDa) with high immunogenicity were very effective in inhibiting the growth of two Gram-positive bacteria (S.aureus, B.sub) that were tested. However, they were only moderately effective in inhibiting the growth of the two tested Gram-negative bacteria (P.aeruginosa and E.coli). However, immunodominant proteins of 22 kDa and 32kDa with high immunogenicity, showed slight effectiveness in inhibiting the growth of two; the Gram-positive and Gram-negative bacteria that were tested. To the best of our knowledge, these immunodominant proteins are novel antigens for potent antimicrobial effects against two gram-positive bacteria (S.aureus, B.subtilis and less antimicrobial effect against two gram-negative bacteria (E.coli, P.aeruginosa) that were prepared. [ABSTRACT FROM AUTHOR]

Published

2017

13. Preparative SDS-PAGE Electroelution for Rapid Purification of Alkyl Hydroperoxide Reductase from Helicobacter pylori

Author

T Mohammadian, M Doosti, M Paknejad, F Siavoshi, and S Massarrat

Subjects

Alkyl hydroperoxide reductase, AhpC, Electroelution, Helicobacter pylori, Public aspects of medicine, RA1-1270

Abstract

"nBackground: Alkyl hydroperoxide reductase (AhpC) of Helicobacter pylori is considered as a diagnostic antigen. There­fore, this antigen can be used to detect H. pylori infection by stool immunoassays such as ELISA. The aim of this study was to simplify the AhpC protein purification procedures."nMethods: For whole cell protein extraction, the bacterial cells were ruptured by octly-β-D glucopyranoside. The isolation and purification of AhpC protein were attempted by various techniques including ammonium sulfate precipitation, dialysis, preparative sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and electroelution."nResults:A simple method was used for protein purification AhpC protein. One-dimensional preparative gel electrophoresis allows a single and short purification step; the high resolution capacity of this technique leads to a high level of purity of the protein. Moreover, it avoids contamination by other non-specific proteins which often appear during protein purification by column chromatography."nConclusion: The present method is simple, rapid and makes it possible to preparate AhpC from H. pylori

Published

2010

14. Producción y purificación de la proteína core del virus de la hepatitis C en el sistema de expresión del baculovirus para ensayos biológicos.

Author

Ivonne Rubio, Alba Lucía Cómbita, Blanca Ortiz Reyes, and María Cristina Navas

Subjects

hepatitis C Virus, core protein, baculovirus, expression system, isoelectrofocusing, electroelution, Medicine, Arctic medicine. Tropical medicine, RC955-962

Abstract

Introducción. La infección por el virus de la hepatitis C (VHC) se caracteriza por la alta frecuencia de infección persistente. La capacidad del VHC para inducir alteraciones en la función de las células del sistema inmune, específicamente en las células dendríticas, parece ser una de las estrategias virales implicada en el establecimiento de la infección persistente. Esta estrategia parece estar mediada en gran parte por una de las proteínas estructurales codificada por el genoma del VHC, la proteína Core, unidad estructural de la cápside viral. Objetivo. Una de las limitantes para la evaluación de las propiedades de Core es la obtención y la purificación de la proteína nativa (191 aa). El objetivo de este estudio fue la producción y la purificación de la proteína Core completa en un sistema eucariote para evaluar las propiedades de la proteína en cultivos de células dendríticas humanas. Resultados. En este estudio se logró la producción de la proteína Core completa en el sistema de expresión de baculovirus y su purificación por la técnica de separación por punto isoeléctrico y electroelución. La pureza de la proteína obtenida se confirmó por Western blot y tinción con plata. Estos análisis mostraron dos bandas únicas correspondientes a las isoformas p23 y p21 de la proteína Core, previamente descritas en la literatura. Conclusiones. La proteína obtenida posee varias de las condiciones de la proteína Core nativa, como peso molecular, isoformas y localización subcelular. Los procedimientos descritos en este artículo son aplicables a proteínas asociadas a membranas producidas en sistemas de expresión eucarióticos.

Published

2005

15. Analysis of Biological Functions of a 60-kD IgE-Binding Component Derived from Sera of Patients with Atopic Dermatitis

Author

J. Bujanowski-Weber, A. Fischer, and W. König

Subjects

Messenger RNA, biology, medicine.diagnostic_test, Cell adhesion molecule, Chemistry, Immunology, CD23, General Medicine, Immunoglobulin E, Flow cytometry, Sepharose, Affinity chromatography, Electroelution, biology.protein, medicine, Immunology and Allergy

Abstract

CD23 and its soluble components (sCD23) play an important role in IgE regulation. Sera of patients with atopic dermatitis (AD) were reported to contain an IgE-binding component with a molecular weight of 60 kD. The aim of our study was to analyze the biological functions of the 60-kD component. Sera of patients with AD were fractionated by ammoniumsulfate precipitation, gel filtration, affinity chromatography on IgE-Sepharose or anti-CD23 Sepharose and electroelution from SDS/PAGE. The sCD23-containing preparations were used in cell culture experiments to stimulate peripheral blood lymphocytes of normal donors. Binding studies with IgE peptides demonstrated that CD23 and the 60-kD IgE-binding components bind to the same site. Further experiments were performed to analyze the induced mRNA pattern in the presence of the 60-kD components by polymerase chain reaction (PCR). These data demonstrated that signals for IgE-germ line transcripts and IFN-γ were induced in the presence of the IgE-binding factor preparations from normal peripheral blood lymphocytes whereas there was no signal obtained for IL-2 or IL-4. In addition, it was shown by flow cytometry that the 60-kD component enhanced the expression of adhesion molecules (CD11α, CD18, CD54) whereas the expression of CD23 was reduced.

Published

2021

16. Sodium dodecyl sulfate free gel electrophoresis/electroelution sorting for peptide fractionation

Author

Luis Javier González, Patricia Sosa-Acosta, Yasset Perez-Riverol, Annia González, Vladimir Besada, Yairet García, Aniel Sanchez, Lila Castellanos-Serra, Yassel Ramos, and Jeovanis Gil

Subjects

Proteomics, Gel electrophoresis, chemistry.chemical_classification, Chromatography, Sodium Dodecyl Sulfate, Filtration and Separation, Peptide, Fractionation, Analytical Chemistry, chemistry.chemical_compound, Electrophoresis, chemistry, Electroelution, Protein purification, Electrophoresis, Polyacrylamide Gel, Sodium dodecyl sulfate, Peptides, Polyacrylamide gel electrophoresis, Chromatography, Liquid

Abstract

Shotgun proteomics based on peptide fractionation by using liquid chromatography has become the common procedure for proteomic studies, although in the very beginning of the field, protein separation by using electrophoresis was the main tool. Nonetheless, during the last two decades, the electrophoretic techniques for peptide mixtures fractionation have evolved as a result of relevant technological improvements. We also proposed the combination of sodium dodecyl sulfate polyacrylamide gel electrophoresis for protein fractionation and sodium dodecyl sulfate free polyacrylamide gel electrophoresis for peptide separation as a novel procedure for proteomic studies. Here, we present an optimized device for sodium dodecyl sulfate free polyacrylamide gel electrophoresis improving peptide recoveries respect to the established electrophoretic technique off gel electrophoresis meanwhile conserving the excellent resolution described for the former technique in slab gel based systems. The device simultaneously allows the separation and the collection of fractionated peptides in solution.

Published

2019

17. RNA electroelution: Comparing two electroeluter models

Author

Amber N. Rogers, Maya K. Mastronardo, Tsion G. Mekonnen, and Ana M. Soto

Subjects

Chromatography, Chemistry, Polyacrylamide, Biophysics, Acrylic Resins, RNA, Cell Biology, Mycobacterium tuberculosis, Biochemistry, Electrophoresis, chemistry.chemical_compound, RNA, Bacterial, Electroelution, Electrophoresis, Polyacrylamide Gel, RNA extraction, Purification methods, Molecular Biology, Polyacrylamide gel electrophoresis, Bacillus subtilis

Abstract

RNA represents a vibrant area of research and many studies use techniques that require large amounts of purified RNA. One common purification method involves slicing a section of a polyacrylamide gel containing the RNA of interest and eluting the RNA out of the gel using electroelution. Various electroeluter models are available but sometimes a given model becomes discontinued, compelling researchers to choose a different model. Here, we have compared two electroeluters with different chamber designs for their ability to recover RNA from gel pieces. Our results show that both electroeluters are effective and recover comparable amounts of purified RNA.

Published

2021

18. Gel Electrophoresis/Electroelution Sorting Fractionator combined with Filter Aided Sample preparation (FASP) for deep proteomic analysis

Author

Yasser Perera, Luis Javier González, Arielis Rodríguez-Ulloa, Yassel Ramos, Almeida A, Carpio J, Wiśniewski, and Besada

Subjects

chemistry.chemical_classification, Gel electrophoresis, Chromatography, Protein mass spectrometry, Chemistry, Electroelution, Proteome, Protein purification, Sample preparation, Peptide, Fractionation

Abstract

Sample preparation and protein fractionation are important issues in proteomic studies in spite of the technological achievements on protein mass spectrometry. Protein extraction procedures strongly affect the performance of fractionation methods by provoking protein dispersion in several fractions. The most notable exception is SDS-PAGE-based protein fractionation due to its extraordinary resolution and the effectiveness of SDS as a solubilizing agent. Its main limitation lies in the poor recovery of the gel-trapped proteins, where protein electro-elution is the most successful approach to overcome this drawback. We created a device to separate complex mixture of proteins and peptides (named “GEES fractionator”) that is based on the continuous Gel Electrophoresis/Electro-elution Sorting of these molecules. In an unsupervised process, complex mixtures of proteins or peptides are fractionated into the gel while separated fractions are simultaneously and sequentially electro-eluted to the solution containing wells. The performance of the device was studied for SDS-PAGE-based protein fractionation in terms of reproducibility, protein recovery and loading capacity. In the SDS-free PAGE setup, complex peptide mixtures can also be fractionated. More than 11 700 proteins were identified in the whole-cell lysate of the CaSki cell line by using the GEES fractionator combined with the Filter Aided Sample Preparation (FASP) method and mass spectrometry analysis. GEES-based proteome characterization shows a 1.7 fold increase in the number of identified proteins compared to the unfractionated sample analysis. Proteins involved in the co-regulated transcription activity, as well as cancer related pathways such as apoptosis signaling, P53 and RAS pathways are more represented in the protein identification output of GEES-based fractionation approaches.

Published

2021

19. Preparation of Chemically Modified DNA Library for SELEX via Incorporation of CLB-dUTP in Primer Extension Reaction.

Author

Puchała M, Radzińska M, Guzdek J, Sok-Grochowska A, Adamowicz-Skrzypkowska A, Pięta P, Jurek P, and Czarnecka M

Subjects

DNA, Single-Stranded, Gene Library, RNA, Aptamers, Nucleotide chemistry, SELEX Aptamer Technique methods

Abstract

Aptamers are single-stranded DNA or RNA molecules which bind with high specificity to the molecular target for which they have been selected. Through a number of unnatural modifications, the diversity of interactions available for this class of molecules can be greatly expanded, potentially leading to better binding properties. Herein we describe a method to prepare an initial chemically modified DNA library for SELEX. It comprises the synthesis of a modified nucleotide in the CuAAC reaction and its purification by an adapted HPLC method. Subsequent stage is the incorporation of the prepared modified nucleotide into a DNA library in a primer extension reaction and a quick and easy method of its purification using an electroelution device. This allows the recovery of the resulting chemically modified ssDNA library with high efficiency to kick off the aptamer selection process., (© 2023. The Author(s), under exclusive license to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2023

20. A reassessment of several erstwhile methods for isolating DNA fragments from agarose gels

Author

Haiyan Zhou, Keyin Zhang, Lucas Zellmer, Tianzhu Lu, Yan Zhao, Yanqin Yu, Dezhong Joshua Liao, Yan He, Hai Huang, and Xia Gao

Subjects

0106 biological sciences, 0301 basic medicine, Review Article, Environmental Science (miscellaneous), 01 natural sciences, law.invention, Dialysis tubing, 03 medical and health sciences, chemistry.chemical_compound, law, Agarose gel, DNA extraction, Polymerase chain reaction, Chromatography, Fragment (computer graphics), Reverse transcription, Agricultural and Biological Sciences (miscellaneous), Reverse transcriptase, 030104 developmental biology, chemistry, Electroelution, Agarose, DNA, 010606 plant biology & botany, Biotechnology, Nested PCR

Abstract

Molecular biology research often requires extraction of DNA fragments from agarose gels. In the past decades, there have been many methods developed for this purpose. Currently most researchers, especially novices, use commercial kits for this extraction, although these kits cost money and the procedures involved are not necessarily easier than some erstwhile methods. We herein reintroduce and reassess several simple and cost-free older methods. One method involves excising a slice of the gel containing the DNA fragment, followed by a thaw-and-freeze procedure to release the DNA from the gel slice into the gel-making buffer. The second method involves a dialysis tubing and requires electroelution of the DNA from the gel slice in the tubing. The third one is to centrifuge the gel slice to release the DNA. The fourth method requires electro-transfer of the DNA from the gel into a filter paper, while the fifth one includes either allowing the DNA in the slice to be dissolved into a buffer or dissolving the DNA-containing gel slice, followed by DNA precipitation with ethanol or isopropanol. The strengths and weaknesses of these methods are discussed to assist researchers in making their choice. We also point out that some of the end uses of the DNA fragment in the agarose gel may not actually require extraction of the DNA. For instance, a tiny DNA-containing gel block or filter paper can be directly used as the template in a nested or semi-nested polymerase chain reaction to preliminarily determine the identity of the DNA fragment.

Published

2021

21. A Native 51 kDa Leishmania Membrane Protein Revealed as a Novel Antigenic Candidate for Immuno-Diagnosis of Human VL and PKDL diseases

Author

Anirban Bhattacharyya, Mohd Kamran, Sarfaraz Ahmad Ejazi, Nicky Didwania, and Nahid Ali

Subjects

Post-kala-azar dermal leishmaniasis, Visceral leishmaniasis, Antigen, Membrane protein, Electroelution, medicine, Biology, medicine.disease, Leishmania, biology.organism_classification, Virology

Published

2020

22. PURIFIKASI PROTEIN IMUNOGENIK 31 DAN 56 kDa DARI KELENJAR SALIVA Aedes aegypti

Author

Fitria Mutiah, Kartika Senjarini, Rike Oktarianti, and Syubbanul Wathon

Subjects

Saliva, biology, Molecular mass, Salivary gland, Chemistry, Dot blot, Aedes aegypti, biology.organism_classification, Molecular biology, Specific antibody, medicine.anatomical_structure, Electroelution, biology.protein, medicine, Antibody

Abstract

Purification of 31 and 56 kDa Immunogenic Protein s from the Salivary Gland s of Aedes aegypti The salivary gland of arthropod vector contains various bioactive compounds and plays a role in the transmission of pathogens to the host. The host develops anti-salivary antibodies against vector saliva exposure. Our previous research has identified two immunogenic proteins with molecular weights of 31 and 56 kDa from the Aedes aegypti salivary gland protein extract. However, the role of the 31 and 56 kDa immunogenic proteins from saliva Ae. aegypti is not fully known, so it is necessary to purify two immunogenic protein fractions to better specify the target of developing a dengue vaccine. This study aimed to purify the 31 and 56 kDa immunogenic protein fractions by electroelution and dialysis methods. The purification of the two protein fractions has been successful which were confirmed by the SDS-PAGE by the existence of single-band parallel to the positive control. These results were further supported by the dot blot analysis which showed a positive reaction in the form of dark spots in the two protein fractions which were reacted with dengue patients' serum, endemic healthy people, and neonates. These results indicated that the purified 31 and 56 kDa immunogenic protein fraction can be identified by specific antibodies . Keywords: dialysis, electroelution, immunogenic, purification, saliva ABSTRAK Kelenjar saliva vektor arthropoda mengandung berbagai senyawa bioaktif dan berperan dalam transmisi patogen ke tubuh inang. Tubuh inang mengembangkan antibodi anti-saliva terhadap paparan saliva vektor. Penelitian kami sebelumnya telah mengidentifikasi dua protein imunogenik dengan berat molekul 31 dan 56 kDa dari ekstrak protein kelenjar saliva Aedes aegypti. Namun demikian, peranan protein imunogenik 31 dan 56 kDa dari saliva Ae . aegypti belum diketahui sepenuhnya sehingga perlu dilakukan purifikasi dua fraksi protein imunogenik untuk lebih menspesifikkan target pengembangan vaksin dengue. Tujuan penelitian ini untuk melakukan purifikasi fraksi protein imunogenik 31 dan 56 kDa melalui metode elektroelusi dan dialisis. Keberhasilan purifikasi dua fraksi protein 31 dan 56 kDa terbukti dari hasil konfirmasi SDS-PAGE dengan terbentuknya pita tunggal sejajar dengan kontrol positif. Hasil tersebut diperkuat dengan analisis dot blot yang menunjukkan reaksi positif dengan munculnya noktah gelap pada dua fraksi protein tersebut ketika direaksikan dengan serum pasien DBD, penduduk sehat endemik dan neonatus. Hasil ini mengindikasikan bahwa fraksi protein imunogenik 31 dan 56 kDa hasil purifikasi dapat dikenali oleh antibodi spesifik.

Published

2020

23. Thermostable Bacteriocin BL8 from Bacillus licheniformis isolated from marine sediment.

Author

Smitha, S. and Bhat, S.G.

Subjects

*BACTERIOCINS, *BACILLUS licheniformis, *MARINE sediments, *GRAM-positive bacteria

Abstract

Aim To isolate and characterize bacteriocin, BL8, from the bacteria identified as Bacillus licheniformis from marine environment. Methods and Results One-hundred and twelve bacterial isolates from sediment and water samples collected off the coast of Cochin, India, were screened for antibacterial activity. Strain BTHT8, identified as Bacillus licheniformis, inhibited the growth of Gram-positive test organisms. The active component labelled as bacteriocin BL8 was partially purified by ammonium sulphate fractionation and was subjected to glycine SDS-PAGE. The band exhibiting antimicrobial activity was electroeluted and analysed using MALDI-TOF mass spectrometry, and the molecular mass was determined as 1·4 kDa. N-terminal amino acid sequencing of BL8 gave a 13 amino acid sequence stretch. Bacteriocin BL8 was stable even after boiling at 100°C for 30 min and over a wide pH range of 1-12. Conclusion A novel, pH-tolerant and thermostable bacteriocin BL8, active against the tested Gram-positive bacteria, was isolated from Bacillus licheniformis. Significance and Impact of the Study This study reports a stable, low molecular weight bacteriocin from Bacillus licheniformis. This bacteriocin can be used to address two important applications: as a therapeutic agent and as a biopreservative in food processing industry. [ABSTRACT FROM AUTHOR]

Published

2013

24. A simple monolithic column electroelution for protein recovery from gel electrophoresis

Author

Li, Guo-Qing, Shao, Jing, Guo, Chen-Gang, Dong, Jing-Yu, Fan, Liu-Yin, and Cao, Cheng-Xi

Subjects

*GEL electrophoresis, *PROTEIN analysis, *PROTEOMICS, *SERUM albumin, *FUNCTIONAL genomics, *MYOGLOBIN

Abstract

Abstract: Protein recovery from gel electrophoresis plays an important role in functional genomics and proteomics but faces a series of issues (e.g., complex procedure, low recovery, long experimental time). In this study, a monolithic column electroelution (MCE) was developed for protein recovery from gel electrophoresis. With the model proteins of bovine serum albumin (BSA), hemoglobin (Hb), and myoglobin (Mb), the developed device and method were compared with common electroelution procedures in agarose gel electrophoresis (AGE). The comparative experiments revealed that (i) the protein recovery achieved with the developed device was greater than 83%, much higher than the 41% to 50% achieved with the common devices; (ii) the running time to obtain 70% recovery was approximately 15min, evidently shorter than the 240min with the common devices; and (iii) the device and procedure were simple and less time-consuming as compared with those of the common devices. It was observed that the serum protein bands cut from polyacrylamide gel electrophoresis could be transferred into solution in 15 to 30min with 82% yield. The device, along with its relevant procedure, has potential use in protein extraction and proteomics as well as in DNA studies. [Copyright &y& Elsevier]

Published

2012

25. Purification and characterization of a thermostable α-amylase produced by the fungus Paecilomyces variotii

Author

Michelin, Michele, Silva, Tony M., Benassi, Vivian M., Peixoto-Nogueira, Simone C., Moraes, Luiz Alberto B., Leão, Juliana M., Jorge, João A., Terenzi, Héctor F., and Polizeli, Maria de Lourdes T.M.

Subjects

*PAECILOMYCES, *CHROMATOGRAPHIC analysis, *SEPHADEX, *AMYLASES, *PULLULANASE, *HYDROLYSIS, *MYCOSES, *CELLULOSE

Abstract

Abstract: An α-amylase produced by Paecilomyces variotii was purified by DEAE-cellulose ion exchange chromatography, followed by Sephadex G-100 gel filtration and electroelution. The α-amylase showed a molecular mass of 75kDa (SDS–PAGE) and pI value of 4.5. Temperature and pH optima were 60°C and 4.0, respectively. The enzyme was stable for 1h at 55°C, showing a t 50 of 53min at 60°C. Starch protected the enzyme against thermal inactivation. The α-amylase was more stable in alkaline pH. It was activated mainly by calcium and cobalt, and it presented as a glycoprotein with 23% carbohydrate content. The enzyme preferentially hydrolyzed starch and, to a lower extent, amylose and amylopectin. The K m of α-amylase on Reagen® and Sigma® starches were 4.3 and 6.2mg/mL, respectively. The products of starch hydrolysis analyzed by TLC were oligosaccharides such as maltose and maltotriose. The partial amino acid sequence of the enzyme presented similarity to α-amylases from Bacillus sp. These results confirmed that the studied enzyme was an α-amylase ((1→4)-α-glucan glucanohydrolase). [ABSTRACT FROM AUTHOR]

Published

2010

26. A method of purification, identification and characterization of β-glucosidase from Trichoderma koningii AS3.2774

Author

Lin, Yuanshan, Chen, Guiguang, Ling, Min, and Liang, Zhiqun

Subjects

*TRICHODERMA, *GLUCOSIDASES, *POLYACRYLAMIDE gel electrophoresis, *ENZYMATIC analysis, *CELLULASE, *SODIUM compounds, *HYDROLASES, *BIOCHEMISTRY technique

Abstract

Abstract: In this study, we used native gradient-polyacrylamide gel electrophoresis and electroelution (NGGEE) to purify enzymatic proteins from Trichoderma koningii AS3.2774. With this method, we purified eight enzymatic proteins and classified them to the cellulase system by comparing secretions of T. koningii in inductive medium and in repressive medium. It resulted in 24-fold β-glucosidase (BG) purification with a recovery rate of 5.5%, and a specific activity of 994.6IUmg−1 protein. The final yield of BG reached 8μg under purifying procedure of NGGEE. We also identified BG using the enzyme assay with thin-layer chromatography and MALDI-TOFMS. This BG had one subunit with a molecular mass of 69.1kDa as determined by sodium dodecylsulfate-polyacrylamide gel electrophoresis. The hydrolytic activity of the BG had an optimal pH of 5.0, an optimal temperature of 50°C, an isoelectric point of 5.68 and a K m for p-nitrophenyl-β-d-glucopyranoside of 2.67mM. Taken together, we show that NGGEE is a reliable method through which μg grade of active proteins can be purified. [Copyright &y& Elsevier]

Published

2010

27. Purification of recombinant growth hormone by clear native gels for conformational analyses: preservation of conformation and receptor binding.

Author

Chen, Wei-Qiang, Salmazo, Anita, Myllykoski, Matti, Sjöblom, Björn, Bidlingmaier, Martin, Pollak, Arnold, Baumgärtel, Peter, Djinovic-Carugo, Kristina, Kursula, Petri, and Lubec, Gert

Subjects

*PROTEIN analysis, *PROTEIN folding, *MONOMERS, *STEREOCHEMISTRY, *PROTEIN conformation

Abstract

Most protein preparations require purification steps prior to biophysical analysis assessing protein stability, secondary structure and degree of folding. It was, therefore, the aim of this study to develop a system to separate and purify a protein from a commercially available medicinal product, recombinant human growth hormone (rhGH) and show preservation of conformation and function following the gel-based procedure. The rhGH was run on clear native (CN) gels and recovered from the gels by electroelution using D-Tube Dialyzer Midi under rigorous cooling. Melting point studies indicated preservation of the structural integrity. This finding was confirmed by synchrotron radiation circular dichroism spectroscopy (SRCD) revealing an identical folding pattern for the sample before and after electrophoretic separation and purification. Synchrotron small-angle X-ray scattering (SAXS) indicated that the sample was folded and monomeric, both before and after separation and purification, and that its shape corresponded well to the known crystal structure of GH. Binding properties of rhGH to a receptor-model system before and after clear native electrophoresis were comparable. This analytical and preparative approach to purify and concentrate a protein preserving conformation and function may be helpful for many applications in analytical, protein and stereochemistry. [ABSTRACT FROM AUTHOR]

Published

2010

28. Adult Brugia malayi ∼34 kDa (BMT-5) antigen offers Th1 mediated significant protection against infective larval challenge in Mastomys coucha

Author

Shakya, Shilpy, Kumar Singh, Prashant, Kushwaha, Susheela, and Misra-Bhattacharya, Shailja

Subjects

*MITOCHONDRIA, *GEL electrophoresis, *LYMPHOPROLIFERATIVE disorders, *IMMUNOREGULATION, *CELL proliferation, *VACCINATION, *MASTOMYS coucha, *NITRIC oxide

Abstract

Abstract: We earlier reported a sizeable protection conferred by ‘mitochondria rich’ (MT) fraction of adult B. malayi and the present study was planned to locate the candidate protective molecule/s in the active fraction. The MT fraction was subjected to sodium dodecyl sulphate polyacrylamide gel electrophoresis (SDS-PAGE) and the antigen bands showing strong immune-reactivity with the resistant mastomys sera were assayed for their lymphoproliferative response using splenocytes of protected animals. Of the eight such protein bands, one sub fraction with a molecular weight of ∼34 kDa (BMT-5) produced utmost cellular proliferation and was therefore exploited for vaccination study. BMT-5 emulsified in Freund''s adjuvant produced discernible protection causing 69 and 67% reductions in microfilaraemia and adult worm burden respectively along with sterilization of 68% of the recovered female parasites. Significant levels of filaria-specific and non-specific lymphoproliferation along with enhanced release of Th1 cytokines (TNF-α, IFN-γ and IL-2) by splenocytes were observed in the vaccinated mastomys in addition to elevated levels of antigen-specific IgG, IgG2a, IgG2b and IgA. The peritoneal macrophages of immunized animals also revealed enhanced nitric oxide production in the presence of BMT-5. The findings suggest that ∼34 kDa (BMT-5) molecules present in the MT fraction of adult B. malayi provided sizeable protection against infective larval challenge by generating a Th1 biased milieu in the host. [Copyright &y& Elsevier]

Published

2009

29. Isolation of High Density Lipoprotein Subclasses by Electrofiltration and Their Chemical Components.

Author

Atmeh, RaghebF., Kana'an, BelalM., and Massad, TariqT.

Subjects

*ELECTROPHORESIS, *HIGH density lipoproteins, *BLOOD lipoproteins, *CHOLESTEROL, *APOLIPOPROTEINS, *LIPIDS

Abstract

The exact role of high density lipoprotein in atheroprotection is not well understood yet due to its complex nature; it comprises more than ten subclasses that vary in size, composition, and function. Isolation and characterization of these subclasses is an important step for further studies addressing their functions in health and disease. In this work, we present a novel method that is relatively simple and efficient for isolation of high density lipoprotein subclasses. The method depends on fractional filtration of the subclasses through a preformed gel membrane system under the effect of an electric field, where the stepwise isolation of the subclasses depends on differences in their rates of migration in polyacrylamide gel. Using this design, we were able to isolate seven high density lipoprotein subclasses with relative molecular masses of 42,000-50,000; 71,000; 103,000; 124,000; 150,000; 182,000; and 219,000. All the subclasses contained apolipoprotein A-I, phosphatidylcholine, sphingomyelin, free cholesterol, esterified cholesterol, and triacylglycerols. Some fractions of some samples contained the apolipoproteins A-II, C-I, C-II, C-III, and E. A subclass of molecular mass of 106,000 was identified and isolated from a healthy young subject that contained albumin and apoA-I with some free and esterified cholesterol, but with no triacylglycerols. This electrofiltration technique offers a novel tool for isolating pure native high density lipoprotein subclasses in a concentrated form that can be used directly for detailed studies of their physicochemical and physiological properties. [ABSTRACT FROM AUTHOR]

Published

2009

30. An improved electroelution method for separation of DNA from humic substances in marine sediment DNA extracts.

Author

Kallmeyer, Jens and Smith, David C.

Subjects

*DNA, *MARINE sediments, *EXTRACTS, *ELECTRIC currents, *ARCHAEBACTERIA, *BIOMASS, *CALCIUM carbonate, *ORGANIC compounds, *MINERALS

Abstract

We present a method for the rapid and simple extraction of DNA from marine sediments using electroelution. It effectively separates DNA from compounds, including humic substances, that interfere with subsequent DNA quantification and amplification. After extraction of the DNA from the sediment into an aqueous solution, the crude sample is encased in 2% agarose gel and exposed to an electrical current, which draws the DNA out of the gel into a centrifugal filter vial. After electroelution, the sample is centrifuged to remove contaminants ≤100 000 Da. Recovery of DNA using this method is quantitative and does not discriminate on the basis of size, as determined using DNA standards and DNA extracts from environmental samples. Amplification of DNA is considerably improved due to removal of PCR inhibitors. For Archaea, only these purified extracts yielded PCR products. This method allows for the use of relatively large volumes of sediment and is particularly useful for sediments containing low biomass such as deeply buried marine sediments. It works with both organic-rich and -poor sediment, as well as with sediment where calcium carbonate is abundant and sediment where it is limited; consequently, adjustment of protocols is unnecessary for samples with very different organic and mineral contents. [ABSTRACT FROM AUTHOR]

Published

2009

31. Impact of seasonal variation on HSP70 expression quantitated in stressed fish hepatocytes

Author

Padmini, Ekambaram and Usha Rani, Munuswamy

Subjects

*HEAT shock proteins, *BIOCHEMICAL variation, *MOLECULAR chaperones, *ENVIRONMENTAL engineering, *ENZYME-linked immunosorbent assay, *OXIDATIVE stress, *ESTUARIES

Abstract

Abstract: Heat shock protein 70 (HSP70) is an effective molecular chaperone, playing a role in cell protection from damage in response to stress stimuli. Here, we report the impact of environmental stress on hepatocyte HSP70 expression in Mugil cephalus living in either a contaminated (Ennore) or uncontaminated (Kovalam) estuary over the course of two seasons. Oxidative and nitrative stress was determined along with quantification of HSP70 by enzyme-linked immunosorbent assay (ELISA) after electroelution from polyacrylamide gels. Fish from Ennore showed significantly higher levels of oxidative and nitrative stress and HSP70 expression than fish from Kovalam. Also, there was significant seasonal variation in all oxidative, nitrative stress marker levels and HSP70 expression which peaked during summer. These results provide direct evidence that HSP70 overexpression in fish hepatocytes under stress may aid cell survival by protecting against oxidative and nitrative stress-induced changes. In addition, seasonal variation may have a significant impact on HSP70 expression. [Copyright &y& Elsevier]

Published

2008

32. A simple and cost-effective method for rapid purification of alkyl hydroperoxide reductase (AhpC) from Helicobacter pylori and its antibody production.

Author

T., Mohammadian, M., Doosti, M., Paknejad, F., Siavoshi, and S., Massarrat

Subjects

*DENATURATION of proteins, *IMMUNOGLOBULINS, *HELICOBACTER pylori, *PEROXIDES, *ANTI-infective agents, *BACTERIAL vaccines

Abstract

Background and the purpose of the study: Helicobacter pylori express abundant amounts of AhpC enzyme that functions to reduce organic hydroperoxides (ROOH) into the corresponding non-toxic alcohols (ROH). This conserved antigen has been earlier described as specific and unique for H. pylori and therefore, both H. pylori AhpC and Anti-AhpC could be useful in the development of serologic and stool antigen tests, to detecting and monitoring H. pylori infection. AhpC may also serves as a potential target for an antimicrobial agent or for vaccine development. The aim of this study was to simplify isolation and purification of the AhpC and production of a highly specific polyclonal antibody against it. Methods and Results: In this paper a simple method was used for protein purification and antibody production which avoids both the long term AhpC protein purification procedure and the addition of Freund's adjuvant. One-dimensional preparative gel electrophoresis allows a single and short purification step and the high resolution capacity of this technique leads to a high level of purity of the protein and consequently to a very high specificity of the antibody. Moreover, it avoids contamination by other non-specific proteins which often appear during protein purification by column chromatographic techniques. Major Conclusion: The present method is simple, rapid and cost-effective and makes it possible to produce antibody for stool antigen enzyme immunoassay in short time and at low cost. [ABSTRACT FROM AUTHOR]

Published

2008

33. Protein complex immunological separation assay (ProCISA): a technique for investigating single protein properties.

Author

Redondo, P., Rosado, J., Salido, G., and Sage, S.

Abstract

Copyright of Journal of Physiology & Biochemistry is the property of Springer Nature 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

2008

34. Separation of biomacromolecules by electrofiltration through gel layers

Author

Atmeh, Ragheb F., Massad, Tariq T., Kana’an, Belal M., and Abu-Alrob, Adam A.

Subjects

*SEPARATION (Technology), *BIOMACROMOLECULES, *POLYACRYLAMIDE, *GEL electrophoresis

Abstract

Abstract: A straightforward method for concomitant separation and isolation of biomacromolecules from a mixture in solution was developed. Three gel layers that comprise a middle separation layer of 10% polyacrylamide gel were constructed. This gel system was formed in an electroconcentration apparatus above a collection chamber surrounded at the bottom by a dialysis membrane. The mixture is applied over the gel layers where biomacromolecules are caused to migrate by electrophoresis through the gel system, where they are separated into discrete bands and electroeluted into the collection chamber without dismantling the apparatus. The isolated biomacromolecules are removed from the chamber in a highly pure and concentrated form ready for further investigations. Cooling can be applied throughout the whole process, and the setup and conditions of run can be modified according to the characteristics of the biomacromolecules to be purified. The components of a mixture containing the glycoprotein ovalbumin and bovine serum albumin monomer, dimer, and tetramer were successfully isolated as concentrated and highly pure fractions with good recoveries ranging from 70 to 89%. Other proteins were successfully isolated under denaturing conditions in the presence of sodium dodecyl sulfate (SDS) or 6M urea. [Copyright &y& Elsevier]

Published

2008

35. In-gel detection of esterase-like albumin activity: Characterization of esterase-free sera albumin and its putative role as non-invasive biomarker of hepatic fibrosis

Author

Riaz Ahmad and Areeba Ahmad

Subjects

Electrophoresis, 0301 basic medicine, Chemistry(all), General Chemical Engineering, Serum albumin, Esterase, Urea denaturation, lcsh:Chemistry, 03 medical and health sciences, Peptide mass fingerprinting, N′-Nitrosodimethylamine, medicine, Hypoalbuminemia, Bovine serum albumin, 030102 biochemistry & molecular biology, biology, Chemistry, Albumin, General Chemistry, medicine.disease, Blood proteins, 030104 developmental biology, lcsh:QD1-999, Biochemistry, Electroelution, Chemical Engineering(all), biology.protein, Hepatic fibrosis, Esterase-like albumin activity

Abstract

Albumin is a globular and un-glycosylated multifunctional plasma protein and thus correlated with several human diseases. Owing to esterase contamination, albumin levels are usually misleading. In this study, we propose methodical accuracy for albumin estimation taking healthy and fibrotic rats. Liver fibrosis in rats was generated by N′-Nitrosodimethylamine (NDMA) (10mg/kg body weight) within three weeks followed by its confirmation through H&E and immunohistochemical staining for α-SMA expression. Animal sera were screened by native polyacrylamide gel electrophoresis (native-PAGE) (7.5%). In-gel esterase-like albumin activity was detected using α- and β-naphthyl acetate (5.58×10−3mM; pH 7.5) as substrate. Sera albumin was purified from unstained PA gel-slices through electroelution. Subsequent to conformation of albumin purity by its molecular weight determination using SDS–PAGE (10%) and peptide mass fingerprinting by MALDI-TOF-MS, samples were treated with different concentrations of urea. Urea-treated albumins were screened for esterase activity, conformational change and, albumin levels by immunoblotting. Our results demonstrate that esterase-like albumin activity in rat sera albumin is located in domain-III. The esterase-like activity remains detectable up to 4M urea, which diminishes with increasing urea concentrations. Further, immunoblotting of urea-treated albumin samples displays a significant decline in purified protein bands, indicating hypoalbuminemia during hepatic fibrosis in rats. In conclusion, the present approach of albumin separation and estimation is of potential interest and may be recommended for diagnostic purposes.

Published

2017

36. Electroelution of lipoprotein(a) [Lp(a)] from native polyacrylamide gels: A new, simple method to purify Lp(a)

Author

Chellan, Bijoy, Appukuttan, P.S., and Jayakumari, N.

Subjects

*BLOOD lipoproteins, *GEL electrophoresis, *ELECTROPHORESIS, *POLYACRYLAMIDE

Abstract

Abstract: Lipoprotein(a), Lp(a), is an atherogenic lipoprotein consisting of an LDL like core particle and a covalently linked glycoprotein of variable size. Lp(a), isolated from serum always contains LDL and HDL2 as contaminants since Lp(a) floats in the density range 1.05–1.12 g/ml which overlaps that of LDL and HDL2. Purified Lp(a) is increasingly needed as a standard to overcome various problems in the standardization of Lp(a) measurements and for in vitro biological studies. Problems inherent to the purification of Lp(a) include the aggregation of Lp(a) with LDL, overlapping size distribution and the inability of some fractions to bind to affinity columns. Here, we describe the development of a new method to purify Lp(a) from contaminating LDL and HDL2 particles. Lp(a) was isolated from serum by sequential ultracentrifugation, resolved by native polyacrylamide gel electrophoresis and the gel segments were electroeluted to obtain pure Lp(a). l-Proline was added to the sample to a final concentration of 0.1 M to prevent the aggregation of Lp(a) with LDL. [Copyright &y& Elsevier]

Published

2006

37. Antibacterial Activity of Isolated Immunodominant Proteins of Naja Naja (Oxiana) Venom

Author

talebi mehrdar, Mahboobeh, madani, Rasool, hajihosseini, Reza, and moradi bidhendi, Soheila

Subjects

Immunodominant protein, Antibacterial effect, Naja Naja, Original Article, complex mixtures, Electroelution

Abstract

The aim of this study is to investigate antibacterial effects of immunodominant proteins isolated from the venom of Naja Naja Oxiana snake against Staphylococcus aureus, Escherichia coli, Bacillus subtilis and Pseudomonas aeruginosa. The innate immune system is an important line of defense against bacterial diseases. Antibacterial peptides and proteins produced by snake venoms have recently attracted significant attention due to their relevance to bacterial diseases and the potential of being converted into new therapeutic agents. Identification of immunodominant proteins of the venom of Naja Naja Oxiana snake was performed by SDS-PAGE and western blot analysis. Identified proteins were isolated directly from preparative gel electrophoresis by Electro-elution. In the next step, antibacterial effects of immunodominant proteins were tested against several strains of clinical isolates, including S.aureus, B.subtilis (Gram-positive bacteria) P.aeruginosa and E.coli (Gram-negative bacteria) using broth microdilution and disc-diffusion assays. In order to compare the results of the disc-diffusion assay, antibacterial effects of several antibiotics (Gentamicin, Ampicillin, Penicillin, Amoxicillin and Ciprofloxacin) were also examined using the same conditions. Results showed that immunodominant proteins of (14, and 65kDa) with high immunogenicity were very effective in inhibiting the growth of two Gram-positive bacteria (S.aureus, B.sub) that were tested. However, they were only moderately effective in inhibiting the growth of the two tested Gram-negative bacteria (P.aeruginosa and E.coli). However, immunodominant proteins of 22 kDa and 32kDa with high immunogenicity, showed slight effectiveness in inhibiting the growth of two; the Gram-positive and Gram-negative bacteria that were tested. To the best of our knowledge, these immunodominant proteins are novel antigens for potent antimicrobial effects against two gram-positive bacteria (S.aureus, B.subtilis ) and less antimicrobial effect against two gram-negative bacteria (E.coli, P.aeruginosa) that were prepared .

Published

2017

38. Enhanced protein recovery after electrotransfer using square wave alternating voltage

Author

Bienvenut, Willy V., Déon, Catherine, Sanchez, Jean-Charles, and Hochstrasser, Denis F.

Subjects

*PROTEINS, *MASS spectrometry

Abstract

Protein identification is becoming a complement to the available fully sequenced genomes. To meet the challenge, newly developed techniques for high throughput protein identification using matrix-assisted laser desorption/ionisation mass spectrometry (MALDI-MS) and peptide mass fingerprint are needed. Two years ago, a parallel protein digestion process was proposed. It provided a collecting polyvinylidene difluoride (PVDF) membrane able to be scanned by MALDI. Acquired data were used to recreate a virtual multidimensional image. Voltage used during this protein electroblotting technique was an unusual square wave alternative voltage (SWAV). The goal of the current study is to evaluate quantitatively the efficiency of the SWAV compared with a classical electroblot process on intact proteins. The effect of the pulsed electric field and the buffer composition were compared to a standard continuous transblotting process defined as the gold standard. Combination of the pulsed asymmetric electric field with 3-(cyclohexylamino)-1-propane-sulfonique acid (CAPS) buffers showed an average 65% increase of protein recovery. Moreover, a strongest effect is observed for high Mr proteins. In conclusion, the present study highlighted a positive influence of the “shaking” effect of the asymmetric alternative voltage on gel protein extraction. [Copyright &y& Elsevier]

Published

2002

39. Expression and purification of recombinant coat protein of sugarcane mosaic virus from Indonesian isolate as an antigen for antibody production

Author

Nurmalasari Darsono, Widhi Dyah Sawitri, Sri Puji Astuti, Natalia Tri Astuti, Suvia Widyaningrum, and Win Darmanto

Subjects

Expression vector, Potyviridae, Potyvirus, antigen, cDNA, recombinant coat protein, sugarcane mosaic virus (SCMV), Environmental Science (miscellaneous), Biology, medicine.disease_cause, biology.organism_classification, Agricultural and Biological Sciences (miscellaneous), Microbiology, law.invention, Sugarcane mosaic virus, law, Electroelution, Complementary DNA, medicine, Recombinant DNA, Escherichia coli, Food Science, Biotechnology

Abstract

Sugarcane mosaic virus (SCMV, genus Potyvirus, family Potyviridae) is a prominent pathogen of sugarcane (Saccharum sp. hybrids). It can cause losses in susceptible varieties, in crop as well as sugar production, economically. Although it has been studied in major sugar-producing countries, research on the definement of SCMV from Indonesian isolates based on molecular study has been very limited. This study aimed to obtain a proper recombinant antigens emanating from coat protein of SCMV from Indonesian isolate in order to produce polyclonal antibodies that cann be used for immunodiagnosis assays in a subsequent study. A gene-encoding coat protein of SCMV (CP-SCMV) was amplified using RT-PCR and cloned into vector pJET1.2. The cDNA was inserted into 6X His-tag expression plasmid of pET28a(+) and over-expressed in Escherichia coli BL21(DE3) to produce a recombinant protein. The highest expression was found in 0.1M IPTG induction media for 5 h at 37oC. SDS-PAGE analysis clarified that the recombinant CP-SCMV remained as an insoluble fraction. Purifications was carried out by the affinity Ni-NTA resin, followed by electroelution to obtain a highly purified protein. To meet the quality requirements of a proper antigen, the highly purified protein was concentrated. A molecular weight of the rCP-SCMV (approximately 40 kDa) was clearly observed by 10% SDS-PAGE at the concentration of 16.184 mg/mL.

Published

2019

40. AgarFix: Simple and accessible stabilization of challenging single-particle cryo-EM specimens through crosslinking in a matrix of agar

Author

Sarah N. Le, Hans Elmlund, Klaudia Adamus, Marion Boudes, and Dominika Elmlund

Subjects

food.ingredient, Materials science, Cryo-electron microscopy, 030303 biophysics, Size-exclusion chromatography, macromolecular substances, Dissociation (chemistry), Specimen Handling, 03 medical and health sciences, chemistry.chemical_compound, Protein Aggregates, food, Structural Biology, Agar, 030304 developmental biology, 0303 health sciences, Drop (liquid), Sepharose, 030302 biochemistry & molecular biology, Cryoelectron Microscopy, Proteins, Reproducibility of Results, Negative stain, Single Molecule Imaging, Sample quality, Cross-Linking Reagents, chemistry, Chemical engineering, Electroelution, Agarose, Macromolecule

Abstract

Cryogenic electron microscopy (cryo-EM) allows structure determination of macromolecular assemblies that have resisted other structural biology approaches because of their size and heterogeneity. These challenging multi-protein targets are typically susceptible to dissociation and/or denaturation upon cryo-EM grid preparation, and often require cross-linking prior to freezing. Several approaches for gentle on-column or in-tube crosslinking have been developed. On-column cross-linking is not widely applicable because of the poor separation properties of gel filtration techniques. In-tube crosslinking frequently causes sample aggregation and/or precipitation. Gradient-based cross-linking through the GraFix method is more robust, but very time-consuming and necessitates specialised expensive equipment. Furthermore, removal of the glycerol typically involves significant sample loss and may cause destabilization detrimental to the sample quality. Here, we introduce an alternative procedure: AgarFix (Agarose Fixation). The sample is embedded in an agarose matrix that keeps the molecules separated, thus preventing formation of aggregates upon cross-linking. Gentle cross-linking is accomplished by diffusion of the cross-linker into the agarose drop. The sample is recovered by diffusion or electroelution and can readily be used for cryo-EM specimen preparation. AgarFix requires minimal equipment and basic lab experience, making it widely accessible to the cryo-EM community.Graphical abstractHighlightsFragile protein complexes can be cross-linked while embedded in agaroseThe agarose matrix prevents formation of aggregates upon cross-linkingCross-linking in agarose is easy, fast, and requires no expensive equipmentThe sample can directly be used for negative stain or cryo-EM grid preparation

Published

2019

41. RNA electroelution: Comparing two electroeluter models.

Author

Rogers, Amber N., Mastronardo, Maya K., Mekonnen, Tsion G., and Soto, Ana Maria

Subjects

*RNA

Abstract

RNA represents a vibrant area of research and many studies use techniques that require large amounts of purified RNA. One common purification method involves slicing a section of a polyacrylamide gel containing the RNA of interest and eluting the RNA out of the gel using electroelution. Various electroeluter models are available but sometimes a given model becomes discontinued, compelling researchers to choose a different model. Here, we have compared two electroeluters with different chamber designs for their ability to recover RNA from gel pieces. Our results show that both electroeluters are effective and recover comparable amounts of purified RNA. [Display omitted] • Electroelution is an efficient and fast way to elute RNA from gel pieces. • Two electroeluters with different cell geometries are similarly successful at eluting RNA out of gel pieces. • Other methods can elute RNA too but passive elution methods may result in RNA degradation, perhaps due to long elution times. [ABSTRACT FROM AUTHOR]

Published

2021

42. Microfluidic chip for stacking, separation and extraction of multiple DNA fragments

Author

Ruige Wu, Y.P. Seah, and Zhiping Wang

Subjects

Gel electrophoresis of nucleic acids, Microfluidics, Analytical chemistry, 02 engineering and technology, Polymerase Chain Reaction, 01 natural sciences, Biochemistry, Analytical Chemistry, chemistry.chemical_compound, Lab-On-A-Chip Devices, Molecular Biology, Oligonucleotide Array Sequence Analysis, Gel electrophoresis, Chromatography, Isotachophoresis, Chemistry, 010401 analytical chemistry, Organic Chemistry, Extraction (chemistry), DNA, General Medicine, 021001 nanoscience & nanotechnology, 0104 chemical sciences, genomic DNA, Electroelution, 0210 nano-technology

Abstract

A disposable integrated microfluidic device was developed for rapid sample stacking, separation and extraction of multiple DNA fragments from a relatively large amount of sample. Isotachophoresis hyphenated gel electrophoresis (ITP-GE) was used to pre-concentrate and separate DNA fragments, followed by extraction of pure DNA fragments with electroelution on-chip. DNA fragments of 200bp, 500bp and 1kbp were successfully separated and collected in the extraction chamber within 25min. The extraction efficiency obtained from the chip was 49.9%, 52.1% and 53.7% for 200bp, 500bp and 1kbp DNA fragments, respectively. The extracted DNA fragments exhibited compatibility with downstream enzymatic reactions, for example PCR. The chip was also used to extract DNA fragments with specific size range from sheared genomic DNA and demonstrated similar performance to that using traditional gel cutting method. The whole assay can finish in 32min, 6 times faster than traditional method.

Published

2016

43. Expression, purification and production of antisera against recombinant truncated VP22 protein

Author

Xian Yu, Zhengmin Xu, Yan Wang, Jun Lei, and Qin Yang

Subjects

0301 basic medicine, Cancer Research, purification, antisera, Immunofluorescence, medicine.disease_cause, law.invention, 03 medical and health sciences, Immunology and Microbiology (miscellaneous), Western blot, law, expression, medicine, Antiserum, medicine.diagnostic_test, biology, Articles, General Medicine, Molecular biology, 030104 developmental biology, Herpes simplex virus, Polyclonal antibodies, Electroelution, biology.protein, Recombinant DNA, VP22, Antibody

Abstract

Cell-penetrating peptides (CPPs) are non-invasive vectors that can efficiently transport bioactive cargo across the cell membrane. Naturally occurring CPPs, such as the tegument protein VP22 of the Herpes simplex virus type 1, can potentiate protein-drug delivery into living cells. The aim of the present study was to construct anti-VP22 antibodies that can be used to detect VP22-fusion drugs. Therefore, 60- and 45-amino acid peptides corresponding to the N-terminus and C-terminus of VP22, respectively, were cloned, expressed and purified. Subsequently, polyclonal antisera against them were generated. The DNA sequence, cloned into the pGEX-5X-1 vector, was transformed into E. coli BL21 (DE3). After inducing expression with 1 mM isopropyl-β-d-thiogalactopyranoside (IPTG) at 25°C for 4 h, the recombinant VP22 proteins were purified by electroelution. The high titers of polyclonal antisera obtained subsequent to immunization of mice with the purified recombinant truncated VP22 was confirmed by ELISA. Western blot and immunofluorescence analysis showed that the antisera detected both the truncated and full-length VP22 protein. Therefore, the polyclonal antisera against VP22 may be used in the detection of the intracellular location of VP22-fusion protein drugs.

Published

2016

44. Characterization of a trypsin-like protease 1 produced by a probiotic Lactobacillus plantarum subsp. plantarum PTCC 1896 from skimmed milk based medium

Author

Mahmoud Sheikh-Zeinoddin, Sabihe Soleimanian-Zad, and Muhannad Haj Mustafa

Subjects

0106 biological sciences, food.ingredient, medicine.medical_treatment, 01 natural sciences, law.invention, Probiotic, 0404 agricultural biotechnology, food, law, 010608 biotechnology, Skimmed milk, medicine, Food science, Protease, biology, Chemistry, food and beverages, 04 agricultural and veterinary sciences, Trypsin, biology.organism_classification, 040401 food science, Electroelution, Fermentation, Bacteria, Lactobacillus plantarum, Food Science, medicine.drug

Abstract

The present study investigates the catalytic activity of a trypsin-like protease (TLP1) and its production management from probiotic bacterium Lactobacillus plantarum subsp. plantarum PTCC 1896. Different culture media were screened for the production of TLP1 at 37 °C. TLP1 was only produced in skimmed milk broth (SMB) medium with the maximal activity of 1.377 ± 0.026 mU/mL following 14 h of fermentation. The optimum temperature and pH for hydrolyzing the trypsin specific substrate N-benzoyl- dl -arginine-p-nitroanilide (BAPNA) were found to be 39 °C and 7.5, respectively. Heat stability of the secreted TLP1 from the bacterium was more than 37 °C, within the pH ranges of 7.0–9.0. The Michaelis–Menten constant (Km) of the filtered TLP1 for BAPNA was 0.8 mM and the maximum velocity was 1.53 pmol/min. The crude TLP1 was purified from SDS-PAGE using the electroelution method. The purified TLP1 showed a single protein band of approximately 25 kDa on SDS-PAGE and 93.3% similar amino acid composition to standard trypsin. Generally, we showed that optimized fermentation conditions can provide sufficient amounts of active and safe TLP1 from the bacterium. The produced TLP1 has great potential to be used for the production of bioactive peptides from natural sources for diabetes prevention.

Published

2020

45. Functional renaturation of receptor polypeptides eluted from SDS polyacrylamide gels.

Author

Hanke, W., Andree, J., Strotmann, J., and Kahle, C.

Abstract

In order to gain further support for the concept that a homo-oligomeric protein-complex may be sufficient to form a functional ligand-activated ion channel and to explore additional possibilities for the reconstitution of channel activity, a single polypeptide band of the purified neuronal AChR from insects has been electroeluted from SDS-polyacrylamide gels, the SDS removed and the polypeptides incorporated into liposomes. Liposomes were fused into planar lipid bilayers which were subsequently analysed for channel activity. Fluctuations of cation-channels were detected after addition of agonists (carbamylcholine); channel activity was blocked by antagonists (d-tubocurarine). The channels formed by electroeluted polypeptides gave conductance values, as well as kinetic data, quite similar to channels formed by the native receptor protein. Sedimentation experiments using sucrose density gradient centrifugation revealed that a considerable portion of the electroeluted polypeptides assembled during the reconstitution process to form oligomeric complexes with a sedimentation coefficient of about 10 S; thus resembling the native receptor complex. [ABSTRACT FROM AUTHOR]

Published

1990

46. Electrophoretic isolation of membrane proteins from acrylamide gels.

Author

Schägger, Hermann

Abstract

Protocols for the optimal resolution of membrane and watersoluble proteins in SDS-denatured state (Tricine SDS-PAGE and Blue Tricine SDS-PAGE; Laemmli SDS-PAGE and Blue Laemmli SDSPAGE) and in the native state (Blue Native PAGE) are presented. The protocols for protein recovery from these gels include techniques of electroelution and electroblotting optimized to the type of the preceding electrophoresis system. Native and denatured proteins thus are obtainable in near quantitative yield in soluble and in immobilized form. These techniques can optionally be performed in the milligram range, e.g., for the use of immunization and N-terminal protein sequencing, or in the analytical range. [ABSTRACT FROM AUTHOR]

Published

1994

47. Monoclonal antibodies used for the characterization of the two putative iron-sulphur centre proteins associated with photosystem I.

Author

Høyer-Hansen, Gunilla, Hønberg, Lisbeth, and Simpson, David

Abstract

Monoclonal antibodies have been produced to the two putative 18.3 and 15.2 kD iron-sulphur centre proteins in barley. When photosystem I particles, containing only chlorophyll a-protein 1 and the 18.3 and 15.2 kD proteins, were used as the antigen, thirteen independent clones secreting either IgG or IgM antibodies against the 15.2 kD protein were formed. No hybridomas secreting antibodies to the 18.3 kD protein were detected. When a delipidated polypeptide preparation was the immunogen, we obtained one hybridoma, secreting antibodies of the IgM class to the 18.3 kD protein. These antibodies were used in immune-blot assays. Neither the 18.3 nor 15.2 kD putative iron-sulphur centre proteins were detected in etioplast membranes. However, in the chloroplast membranes of the photosystem I mutant viridis-zb we found small amounts of these proteins. The two proteins were purified by electroelution and then tested by immune-blot assay. Fractions with positive reaction were collected and the amino acid compositions determined. There were significant differences in the amounts of serine, glycine and histidine between the two proteins. [ABSTRACT FROM AUTHOR]

Published

1985

48. Preparative SDS-PAGE Electroelution for Rapid Purification of Alkyl Hydroperoxide Reductase from Helicobacter pylori.

Author

Mohammadian, T., Doosti, M., Paknejad, M., Siavoshi, F., and Massarrat, S.

Abstract

Background: Alkyl hydroperoxide reductase (AhpC) of Helicobacter pylori is considered as a diagnostic antigen. Therefore, this antigen can be used to detect H. pylori infection by stool immunoassays such as ELISA. The aim of this study was to simplify the AhpC protein purification procedures. Methods: For whole cell protein extraction, the bacterial cells were ruptured by octly-β-D glucopyranoside. The isolation and purification of AhpC protein were attempted by various techniques including ammonium sulfate precipitation, dialysis, preparative sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) and electroelution. Results:A simple method was used for protein purification AhpC protein. One-dimensional preparative gel electrophoresis allows a single and short purification step; the high resolution capacity of this technique leads to a high level of purity of the protein. Moreover, it avoids contamination by other non-specific proteins which often appear during protein purification by column chromatography. Conclusion: The present method is simple, rapid and makes it possible to preparate AhpC from H. pylori. [ABSTRACT FROM AUTHOR]

Published

2010

49. Protein Extraction from Gels: A Brief Review

Author

Rachna Aggarwal, Biji T. Kurien, and R. Hal Scofield

Subjects

chemistry.chemical_classification, 0303 health sciences, Chromatography, Elution, 02 engineering and technology, Gel electrophoresis of proteins, 021001 nanoscience & nanotechnology, 03 medical and health sciences, Electrophoresis, chemistry.chemical_compound, Enzyme, chemistry, Electroelution, Protein purification, Sodium dodecyl sulfate, 0210 nano-technology, Polyacrylamide gel electrophoresis, 030304 developmental biology

Abstract

Protein gel electrophoresis is an important procedure carried out in protein studies. Elution and recovery of proteins separated by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) are often necessary for further downstream analyses. The process involves localizing the protein of interest on the gel following SDS-PAGE, eluting the protein from the gel, removing SDS from the eluted sample, and finally renaturing the protein (e.g., enzymes) for subsequent analyses. Investigators have extracted proteins from gels by a variety of techniques. These include dissolution of the gel matrix, passive diffusion, and electrophoretic elution. Proteins eluted from gels have been used successfully in a variety of downstream applications, including protein chemistry, proteolytic cleavage, determination of amino acid composition, polypeptide identification by trypsin digestion and matrix-assisted laser desorption ionization-time of flight mass spectroscopy, as antigens for antibody production, identifying a polypeptide corresponding to an enzyme activity, and other purposes. Protein yields ranging from nanogram levels to 100 μg have been obtained. Here, we review some of the methods that have been used to elute proteins from gels.

Published

2018

50. Enzymatic Synthesis and Fractionation of Fluorescent PolyU RNAs

Author

Christian Beren, William M. Gelbart, Charles M. Knobler, Katherine N. Liu, and Lisa L. Dreesens

Subjects

Gel electrophoresis, Strategy and Management, Mechanical Engineering, Metals and Alloys, RNA, Industrial and Manufacturing Engineering, Nucleobase, Nucleic acid secondary structure, Uridine diphosphate, chemistry.chemical_compound, Biochemistry, chemistry, Electroelution, Methods Article, Polynucleotide phosphorylase, Nucleic acid structure

Abstract

The physical properties of viral-length polyuridine (PolyU) RNAs, which cannot base-pair and form secondary structures, are compared with those of normal-composition RNAs, composed of comparable numbers of each of A, U, G and C nucleobases. In this protocol, we describe how to synthesize fluorescent polyU RNAs using the enzyme polynucleotide phosphorylase (PNPase) from Uridine diphosphate (UDP) monomers and how to fractionate the polydisperse synthesis mixture using gel electrophoresis, and, after electroelution, how to quantify the amount of polyU recovered with UV-Vis spectrophotometry. Dynamic light scattering was used to determine the hydrodynamic radii of normal-composition RNAs as compared to polyU. It showed that long polyU RNAs behave like linear polymers for which the radii scale with chain length as N(1/2), as opposed to normal-composition RNAs that act as compact, branched RNAs for which the radii scale as N(1/3).

Published

2018