Multi-omics method for single cell transcriptome and translation group combined sequencing

A technology of transcriptome sequencing and transcriptome, applied in biochemical equipment and methods, microbial measurement/inspection, etc., can solve problems such as less protein translation, inability to translate protein translation and transcription linkage at the genome level, and protein level research.

Active Publication Date: 2021-05-25
TSINGHUA UNIV
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Problems solved by technology

However, due to technical bottlenecks, the existing single-cell multi-omics technology mainly focuses on the combination of DNA, mRNA, DNA and chromatin modification, but there are few studies on protein translation or protein level.
Although some research groups have tried to combine the transcriptome and proteome based on antibody-labeled protein antigens, they can only detect dozens of proteins with high abundance, and cannot link translation and transcription of proteins at the genome-wide level. to study together

Method used

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  • Multi-omics method for single cell transcriptome and translation group combined sequencing
  • Multi-omics method for single cell transcriptome and translation group combined sequencing
  • Multi-omics method for single cell transcriptome and translation group combined sequencing

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Embodiment 1

[0075] 1. Reagent preparation

[0076] 1. Polysome buffer

[0077] 20mM Tris-HCl, pH=7.4

[0078] 150mM NaCl

[0079] 5mM MgCl 2

[0080] 1mM DTT

[0081] 100 μg / mL CHX

[0082] 2. Lysis solution

[0083] 1× polysome buffer

[0084] 1% by mass Triton-X 100

[0085] 25U / mL Turbo DNase

[0086] 3. Sucrose buffer solution

[0087] 1× polysome buffer

[0088] 1M sucrose

[0089] 20U / mL SUPERase.In

[0090] 4. RNA gel extraction buffer

[0091] 300mM sodium acetate, pH 5.5

[0092] 0.25% by mass SDS

[0093] 1 mM EDTA

[0094] 5. Clumping buffer

[0095] 1% by mass SDS

[0096] 10mM Tirs, pH=7.5

[0097] 2. Preparation of cell lysate

[0098] 1. Place the cell sample at the bottom of a 1.5 mL RNase / DNase-free EP tube, and the volume of the liquid contained should not exceed 2 μL.

[0099] 2. Add 20 μL of ice-cold lysis buffer to the sample, shake slightly, incubate the centrifuge tube on ice for 10 minutes, centrifuge, and collect the supernatant.

[0100] 3. ...

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Abstract

The invention provides a method for simultaneously carrying out transcriptome sequencing and transscriptome sequencing, which is characterized by comprising the following steps: carrying out first-step lysis treatment on cells and a lysis buffer solution to obtain a first lysis solution; after uniformly mixing and centrifuging, taking a part of the first lysis solution in the supernate as a transcriptome template, and taking the rest of the supernate and the lysis buffer solution to carry out second lysis treatment so as to obtain a second lysis solution; centrifuging the second lysate, and collecting supernate as a translation group template; obtaining a transcriptome cDNA library by using the transcriptome template, and sequencing the transcriptome cDNA library; and extracting a ribosome protected RNA fragment from the translation group template, and carrying out library establishment and sequencing on the ribosome protected RNA fragment. According to the method, high-quality transcriptome and translation group data in a whole genome range can be obtained at the same time, and the method is particularly suitable for single cells, so that possibility is provided for knowing collaborative regulation of single cell transcription and translation levels.

Description

technical field [0001] The present invention relates to the field of biology. In particular, the present invention relates to methods for performing transcriptome sequencing and translationome sequencing simultaneously. Background technique [0002] In recent years, with the development of next-generation sequencing technology, the emergence of many high-throughput sequencing technologies is helping people gain an in-depth understanding of various processes in biology. For research related to gene expression regulation, a large number of omics technologies based on the measurement of DNA and mRNA levels have emerged. Among them, the single-cell transcriptome method was first established in 2009, has undergone a series of optimizations, and has been widely used in various biological research processes today. However, single-cell transcriptome sequencing cannot accurately reflect the abundance of proteins encoded by each gene in the cell, because the translation efficiency a...

Claims

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Application Information

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Patent Type & Authority Applications(China)
IPC IPC(8): C12Q1/6869
CPCC12Q1/6869C12Q2521/345C12Q2527/125C12Q2527/127C12Q2521/327C12Q2531/113C12Q2521/107C12Q2565/125C12Q1/68
Inventor 颉伟熊竹清邹卓宁
Owner TSINGHUA UNIV
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