SPRINT: a Cas13a-based platform for detection of small molecules

被引:60
作者
Iwasaki, Roman S. [1 ]
Batey, Robert T. [1 ]
机构
[1] Univ Colorado, Dept Biochem, Boulder, CO 80309 USA
基金
美国国家卫生研究院;
关键词
PURINE-NUCLEOSIDE PHOSPHORYLASE; NUCLEIC-ACID DETECTION; IN-VITRO SELECTION; LIGAND-BINDING; SYNTHETIC RIBOSWITCH; BACILLUS-SUBTILIS; RNA; ANALOGS; TRANSCRIPTION; RECOGNITION;
D O I
10.1093/nar/gkaa673
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
Recent efforts in biological engineering have made detection of nucleic acids in samples more rapid, inexpensive and sensitive using CRISPR-based approaches. We expand one of these Cas13a-based methods to detect small molecules in a one-batch assay. Using SHERLOCK-based profiling of in vitro transcription (SPRINT), in vitro transcribed RNA sequence-specifically triggers the RNase activity of Cas13a. This event activates its non-specific RNase activity, which enables cleavage of an RNA oligonucleotide labeled with a quencher/fluorophore pair and thereby de-quenches the fluorophore. This fluorogenic output can be measured to assess transcriptional output. The use of riboswitches or proteins to regulate transcription via specific effector molecules is leveraged as a coupled assay that transforms effector concentration into fluorescence intensity. In this way, we quantified eight different compounds, including cofactors, nucleotides, metabolites of amino acids, tetracycline and monatomic ions in samples. In this manner, hundreds of reactions can be easily quantified in a few hours. This increased throughput also enables detailed characterization of transcriptional regulators, synthetic compounds that inhibit transcription, or other coupled enzymatic reactions. These SPRINT reactions are easily adaptable to portable formats and could therefore be used for the detection of analytes in the field or at point-of-care situations.
引用
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页数:16
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