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胞嘧啶脱氨酶的发现使得利用单一酶进行碱基分辨率甲基化组图谱绘制成为可能。

Discovery of cytosine deaminases enables base-resolution methylome mapping using a single enzyme.

作者信息

Vaisvila Romualdas, Johnson Sean R, Yan Bo, Dai Nan, Bourkia Billal M, Chen Minyong, Corrêa Ivan R, Yigit Erbay, Sun Zhiyi

机构信息

New England Biolabs Inc., 240 County Road, Ipswich, MA 01938, USA.

New England Biolabs Inc., 240 County Road, Ipswich, MA 01938, USA.

出版信息

Mol Cell. 2024 Mar 7;84(5):854-866.e7. doi: 10.1016/j.molcel.2024.01.027. Epub 2024 Feb 22.

Abstract

Deaminases have important uses in modification detection and genome editing. However, the range of applications is limited by the small number of characterized enzymes. To expand the toolkit of deaminases, we developed an in vitro approach that bypasses a major hurdle with their toxicity in cells. We assayed 175 putative cytosine deaminases on a variety of substrates and found a broad range of activity on double- and single-stranded DNA in various sequence contexts, including CpG-specific deaminases and enzymes without sequence preference. We also characterized enzyme selectivity across six DNA modifications and reported enzymes that do not deaminate modified cytosines. The detailed analysis of diverse deaminases opens new avenues for biotechnological and medical applications. As a demonstration, we developed SEM-seq, a non-destructive single-enzyme methylation sequencing method using a modification-sensitive double-stranded DNA deaminase. The streamlined protocol enables accurate, base-resolution methylome mapping of scarce biological material, including cell-free DNA and 10 pg input DNA.

摘要

脱氨酶在修饰检测和基因组编辑中具有重要用途。然而,应用范围受到已表征酶数量较少的限制。为了扩展脱氨酶的工具集,我们开发了一种体外方法,绕过了它们在细胞中的毒性这一主要障碍。我们在多种底物上检测了175种假定的胞嘧啶脱氨酶,发现在各种序列背景下,包括CpG特异性脱氨酶和无序列偏好的酶,它们对双链和单链DNA都具有广泛的活性。我们还表征了六种DNA修饰的酶选择性,并报道了不会使修饰胞嘧啶脱氨的酶。对多种脱氨酶的详细分析为生物技术和医学应用开辟了新途径。作为一个示范,我们开发了SEM-seq,一种使用修饰敏感双链DNA脱氨酶的非破坏性单酶甲基化测序方法。简化的方案能够对包括游离DNA和10 pg输入DNA在内的稀缺生物材料进行准确的碱基分辨率甲基化组图谱绘制。

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