国产精口品美女乱子伦高潮-亚洲日本中文字幕网站-激情国产AV做激情国产爱-丰满少妇被猛男猛烈进入久久

新聞動態(tài) News
聯(lián)系方式 Contact

地址:廈門市集美大道1300號

電話:15805933710

聯(lián)系人:許先生

QQ:1974707632 (節(jié)假日可詢)

微信:15805933710 (節(jié)假日可詢)

郵件:purimag@139.com

在線QQ交談 在線QQ交談

搜索 Search

客戶采用我司SA磁珠篩選適配體在《Sensors and Actuators B: Chemical》發(fā)文

2021-6-2 21:16:58點擊:


客戶采用我司SA磁珠(PuriMag G-NH2)偶聯(lián)PD-L1篩選適配體。


Hongwei Hu, Yujing Ding, Zihan Gao, Hao Li,
S1 nuclease digestion-based rational truncation of PD-L1 aptamer and establishment of a signal dual amplification aptasensor,
Sensors and Actuators B: Chemical,
Volume 331,
2021,
129442,
ISSN 0925-4005,
https://doi.org/10.1016/j.snb.2021.129442.
(http://www.sciencedirect.com.group21-s.aronip.com/science/article/pii/S0925400521000101)


Abstract: Truncation optimization of aptamers can improve both specificity and robustness. At present, aptamer truncation is mainly performed based on predictions from molecular docking simulations, but this usually requires tedious trial-and-error and may result in false predictions. Here, we propose a strategy based on digestion by S1 nuclease to rationally truncate the aptamer, using the PD-L1-binding aptamer Apt80 as an example. Due to steric hindrance, recognition and binding regions between Apt80 and PD-L1 are not digested by the enzyme. The truncated form, Apt38, shows higher affinity and larger conformational change after binding, when compared to Apt80. The truncated Apt38 was used as a platform for developing a signal dual ampli?cation fluorescence aptasensor using targeted recycling assisted by exonuclease I and qRT-PCR analysis. This aptasensor exhibited a high sensitivity toward PD-L1 with a limit of detection of 0.076 ng/mL in buffer system and 0.3625 ng/mL in human serum. Owing to its high sensitivity, specificity, ease operation and low cost for detection of PD-L1, this aptasensor should be useful in assisting clinicians to evaluate the status of cancer patient and to decide whether inhibitor drugs are needed.
Keywords: Aptamer truncation; S1 nuclease digestion; PD-L1; Signal dual amplification aptasensor

摘要:核酸適體的截短優(yōu)化可以提高其特異性和魯棒性。目前,核酸適體的截短主要是基于分子對接模擬的預(yù)測,但這通常需要繁瑣的試錯,并可能導(dǎo)致錯誤的預(yù)測。本文以PD-L1結(jié)合適體Apt80為例,提出了一種基于S1核酸酶消化的策略來合理截斷適體。由于空間位阻,Apt80和PD-L1之間的識別和結(jié)合區(qū)域不能被酶消化。與Apt80相比,截短的Apt38在結(jié)合后表現(xiàn)出更高的親和力和更大的構(gòu)象變化。截短的Apt38被用作開發(fā)信號雙擴增熒光aptasensor的平臺,利用核酸外切酶I和qRT-PCR分析輔助靶向回收。該傳感器對PD-L1具有較高的靈敏度,在緩沖體系中的檢出限為0.076ng/mL,在人血清中的檢出限為0.3625ng/mL。該傳感器具有靈敏度高、特異性強、操作簡便、檢測成本低等優(yōu)點,有助于臨床醫(yī)生對腫瘤患者病情的評估及是否需要使用抑制劑。

關(guān)鍵詞:適體截短;S1核酸酶消化;PD-L1;信號雙放大自適應(yīng)傳感器


更多鏈霉親和素磁珠 http://www.tools.7z1ocr.cn/Product/8271042221.html