Aptameric Probe Specifically Binding Protein Heterodimer Rather Than Monomers

Aptameric Probe Specifically Binding Protein Heterodimer Rather Than Monomers

Abstract Dimerization of proteins occurs frequently and plays integral roles in biological processes. However, no single molecular probe is available for in situ detection of protein dimers on cells and tissues because of the difficulty of isolating complete protein dimers for probe preparation and...

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Main Authors: Tao Bing, Luyao Shen, Junyan Wang, Linlin Wang, Xiangjun Liu, Nan Zhang, Xiao Xiao, Dihua Shangguan
Format: Article
Language:English
Published: Wiley 2019-06-01
Series:Advanced Science
Subjects:
alkaline phosphatase
aptamers
molecular probes
protein heterodimers
recognition
Online Access:https://doi.org/10.1002/advs.201900143
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spelling doaj-3698e4db1b5b46aca7231e49b5b2b2ab2020-11-25T00:28:29ZengWileyAdvanced Science2198-38442019-06-01611n/an/a10.1002/advs.201900143Aptameric Probe Specifically Binding Protein Heterodimer Rather Than MonomersTao Bing0Luyao Shen1Junyan Wang2Linlin Wang3Xiangjun Liu4Nan Zhang5Xiao Xiao6Dihua Shangguan7Beijing National Laboratory for Molecular Sciences Key Laboratory of Analytical Chemistry for Living Biosystems CAS Research/Education Center for Excellence in Molecular Sciences Institute of Chemistry Chinese Academy of Sciences Beijing 100190 ChinaBeijing National Laboratory for Molecular Sciences Key Laboratory of Analytical Chemistry for Living Biosystems CAS Research/Education Center for Excellence in Molecular Sciences Institute of Chemistry Chinese Academy of Sciences Beijing 100190 ChinaBeijing National Laboratory for Molecular Sciences Key Laboratory of Analytical Chemistry for Living Biosystems CAS Research/Education Center for Excellence in Molecular Sciences Institute of Chemistry Chinese Academy of Sciences Beijing 100190 ChinaBeijing National Laboratory for Molecular Sciences Key Laboratory of Analytical Chemistry for Living Biosystems CAS Research/Education Center for Excellence in Molecular Sciences Institute of Chemistry Chinese Academy of Sciences Beijing 100190 ChinaBeijing National Laboratory for Molecular Sciences Key Laboratory of Analytical Chemistry for Living Biosystems CAS Research/Education Center for Excellence in Molecular Sciences Institute of Chemistry Chinese Academy of Sciences Beijing 100190 ChinaBeijing National Laboratory for Molecular Sciences Key Laboratory of Analytical Chemistry for Living Biosystems CAS Research/Education Center for Excellence in Molecular Sciences Institute of Chemistry Chinese Academy of Sciences Beijing 100190 ChinaBeijing National Laboratory for Molecular Sciences Key Laboratory of Analytical Chemistry for Living Biosystems CAS Research/Education Center for Excellence in Molecular Sciences Institute of Chemistry Chinese Academy of Sciences Beijing 100190 ChinaBeijing National Laboratory for Molecular Sciences Key Laboratory of Analytical Chemistry for Living Biosystems CAS Research/Education Center for Excellence in Molecular Sciences Institute of Chemistry Chinese Academy of Sciences Beijing 100190 ChinaAbstract Dimerization of proteins occurs frequently and plays integral roles in biological processes. However, no single molecular probe is available for in situ detection of protein dimers on cells and tissues because of the difficulty of isolating complete protein dimers for probe preparation and screening, which has greatly hampered the biomedical study of protein dimers. Herein, a G‐rich DNA aptamer (termed BG2) that only binds alkaline phosphatase (AP) heterodimers rather than monomers is reported. This aptamer is generated by the cell‐SELEX (systematic evolution of ligands by exponential enrichment) technique and proves to fold into a duplex stabilized antiparallel G‐quadruplex structure. Using BG2 as molecular probe, AP heterodimers are found to be expressed on several kinds of cancer cells. As an affinity ligand, BG2 could isolate AP heterodimers from cell lysate. BG2 is also demonstrated to be applicable for tumor imaging in mice xenografted with cells highly expressing AP heterodimers. AP isozymes are found in several tissues and blood throughout the body, but the function and tissue distribution of AP heterodimers are totally unknown; therefore, BG2 could serve as a molecular probe to uncover the mystery of AP heterodimers. The generation of aptameric probes by cell‐SELEX will open up a new situation for the study of protein dimers.https://doi.org/10.1002/advs.201900143alkaline phosphataseaptamersmolecular probesprotein heterodimersrecognition
collection DOAJ
language English
format Article
sources DOAJ
author Tao Bing
Luyao Shen
Junyan Wang
Linlin Wang
Xiangjun Liu
Nan Zhang
Xiao Xiao
Dihua Shangguan
spellingShingle Tao Bing
Luyao Shen
Junyan Wang
Linlin Wang
Xiangjun Liu
Nan Zhang
Xiao Xiao
Dihua Shangguan
Aptameric Probe Specifically Binding Protein Heterodimer Rather Than Monomers
Advanced Science
alkaline phosphatase
aptamers
molecular probes
protein heterodimers
recognition
author_facet Tao Bing
Luyao Shen
Junyan Wang
Linlin Wang
Xiangjun Liu
Nan Zhang
Xiao Xiao
Dihua Shangguan
author_sort Tao Bing
title Aptameric Probe Specifically Binding Protein Heterodimer Rather Than Monomers
title_short Aptameric Probe Specifically Binding Protein Heterodimer Rather Than Monomers
title_full Aptameric Probe Specifically Binding Protein Heterodimer Rather Than Monomers
title_fullStr Aptameric Probe Specifically Binding Protein Heterodimer Rather Than Monomers
title_full_unstemmed Aptameric Probe Specifically Binding Protein Heterodimer Rather Than Monomers
title_sort aptameric probe specifically binding protein heterodimer rather than monomers
publisher Wiley
series Advanced Science
issn 2198-3844
publishDate 2019-06-01
description Abstract Dimerization of proteins occurs frequently and plays integral roles in biological processes. However, no single molecular probe is available for in situ detection of protein dimers on cells and tissues because of the difficulty of isolating complete protein dimers for probe preparation and screening, which has greatly hampered the biomedical study of protein dimers. Herein, a G‐rich DNA aptamer (termed BG2) that only binds alkaline phosphatase (AP) heterodimers rather than monomers is reported. This aptamer is generated by the cell‐SELEX (systematic evolution of ligands by exponential enrichment) technique and proves to fold into a duplex stabilized antiparallel G‐quadruplex structure. Using BG2 as molecular probe, AP heterodimers are found to be expressed on several kinds of cancer cells. As an affinity ligand, BG2 could isolate AP heterodimers from cell lysate. BG2 is also demonstrated to be applicable for tumor imaging in mice xenografted with cells highly expressing AP heterodimers. AP isozymes are found in several tissues and blood throughout the body, but the function and tissue distribution of AP heterodimers are totally unknown; therefore, BG2 could serve as a molecular probe to uncover the mystery of AP heterodimers. The generation of aptameric probes by cell‐SELEX will open up a new situation for the study of protein dimers.
topic alkaline phosphatase
aptamers
molecular probes
protein heterodimers
recognition
url https://doi.org/10.1002/advs.201900143
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AT nanzhang aptamericprobespecificallybindingproteinheterodimerratherthanmonomers
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