Thymidine Phosphodiester Chemiluminescent Probe for Sensitive and Selective Detection of Ectonucleotide Pyrophosphatase 1.

IF 4 2区化学 Q1 BIOCHEMICAL RESEARCH METHODS

Bioconjugate Chemistry Pub Date : 2025-01-09 DOI:10.1021/acs.bioconjchem.4c00454

Omri Shelef, Sara Gutkin, Molhm Nassir, Anne Krinsky, Ronit Satchi-Fainaro, Phil S Baran, Doron Shabat

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引用次数: 0

Abstract

ENPP-1 is a transmembrane enzyme involved in nucleotide metabolism, and its overexpression is associated with various cancers, making it a potential therapeutic target and biomarker for early tumor diagnosis. Current detection methods for ENPP-1 utilize a colorimetric probe, TMP-pNP, which has significant limitations in sensitivity. Here, we present probe CL-ENPP-1, the first nucleic acid-based chemiluminescent probe designed for rapid and highly sensitive detection of ENPP-1 activity. The design of probe CL-ENPP-1 features a phenoxy-adamantyl-1,2-dioxetane luminophore linked to thymidine via a phosphodiesteric bond. Upon cleavage of the enzymatic substrate by ENPP-1, the probe undergoes an efficient chemiexcitation process to emit a green photon. Probe CL-ENPP-1 demonstrates an exceptional signal-to-noise ratio of 15000 and a limit of detection value approximately 4500-fold lower than the widely used colorimetric probe TMP-pNP. A comparison of TMP-pNP activation by ENPP-1 versus alkaline phosphatase (ALP) reveals a complete lack of selectivity. Removal of the self-immolative spacer from probe CL-ENPP-1 resulted in a new chemiluminescent probe, CL-ENPP-2, with an 18.4-fold increase in selectivity for ENPP-1 over ALP. The ability of probe CL-ENPP-2 to detect ENPP-1 activity in mammalian cells was assessed using the human breast cancer cell line MDA-MB-231. This probe demonstrated a 19.5-fold improvement in the signal-to-noise ratio, highlighting its superior ability to detect ENPP-1 activity in a biological sample. As far as we know, to date, CL-ENPP-1 and CL-ENPP-2 are the most sensitive probes for the detection of ENPP-1 catalytic activity. We anticipate that our new chemiluminescent probes will be valuable for various applications requiring ENPP-1 detection, including enzyme inhibitor-based drug discovery assays. The insights gained from our probe design principles could advance the development of more selective probes for ENPP-1 and contribute to future innovations in chemiluminescence research.

查看原文本刊更多论文

胸苷磷酸二酯化学发光探针灵敏选择性检测外核苷酸焦磷酸酶1。

ENPP-1是一种参与核苷酸代谢的跨膜酶，其过表达与多种癌症有关，是肿瘤早期诊断的潜在治疗靶点和生物标志物。目前的ENPP-1检测方法利用比色探针，TMP-pNP，其灵敏度有很大的局限性。在这里，我们提出了探针CL-ENPP-1，这是第一个基于核酸的化学发光探针，设计用于快速和高灵敏度检测ENPP-1活性。探针CL-ENPP-1的设计特点是一个苯氧基-adamantyl-1,2-二氧基发光团通过磷二酯键与胸腺嘧啶相连。在ENPP-1切割酶底物后，探针经历了一个有效的化学激发过程，发射绿色光子。探针CL-ENPP-1具有15000的特殊信噪比，检测值的极限比广泛使用的比色探针TMP-pNP低约4500倍。通过比较ENPP-1与碱性磷酸酶（ALP）对TMP-pNP的激活，我们发现它们完全缺乏选择性。从探针CL-ENPP-1中去除自牺牲间隔，得到了新的化学发光探针CL-ENPP-2，其对ENPP-1的选择性比ALP提高了18.4倍。利用人乳腺癌细胞系MDA-MB-231检测探针CL-ENPP-2在哺乳动物细胞中检测ENPP-1活性的能力。该探针的信噪比提高了19.5倍，突出了其在生物样品中检测ENPP-1活性的优越能力。据我们所知，迄今为止，CL-ENPP-1和CL-ENPP-2是检测ENPP-1催化活性最敏感的探针。我们预计我们的新化学发光探针将对需要ENPP-1检测的各种应用有价值，包括基于酶抑制剂的药物发现分析。从我们的探针设计原理中获得的见解可以促进更多选择性ENPP-1探针的发展，并有助于未来化学发光研究的创新。

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来源期刊

Bioconjugate Chemistry 生物-化学综合

CiteScore

9.00

自引率

2.10%

发文量

236

审稿时长

1.4 months

期刊介绍： Bioconjugate Chemistry invites original contributions on all research at the interface between man-made and biological materials. The mission of the journal is to communicate to advances in fields including therapeutic delivery, imaging, bionanotechnology, and synthetic biology. Bioconjugate Chemistry is intended to provide a forum for presentation of research relevant to all aspects of bioconjugates, including the preparation, properties and applications of biomolecular conjugates.