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Total RNA Purification Kit

For purification of RNA from cells

Total RNA Purification Kit

For purification of RNA from cells

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For purification of RNA from cells
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What's Included

  • Total RNA Purification Kit (Catalog #79040)
    • RNA Minicolumns, 50x
    • Collection Tubes, 2 x 50
    • Column Wash Solution, 5 mL
    • 1-Thioglycerol, 900 µL
    • DNase I (lyophilized), 1 x 1 vial
    • Nuclease-Free Water, 13 mL
    • MnCl2, 250 µL
    • RNA Lysis Buffer, 32.5 mL
    • Elution Tubes, 50x
    • RNA Wash Solution, 35 mL
    • DNA Digestion Buffer, 2.5 mL
Products for Your Protocol
To see all required products for your protocol, please consult the Protocols and Documentation.

Overview

The Total RNA Purification Kit uses a membrane-based system to quickly purify intact total RNA from 1 x 10^2 to 5 x 10^6 cells without an organic extraction step, eliminating the need for additional purification steps. The Total RNA Purification Kit includes an on-column DNase I treatment to significantly reduce genomic DNA contamination and ensure the purified RNA is suitable for sensitive downstream applications. Intact total RNA can be isolated in as little as 30 minutes. The Total RNA Purification Kit is not recommended for the purification of small RNAs (< 200 nt), such as miRNA
Application
Genome Editing

Protocols and Documentation

Find supporting information and directions for use in the Product Information Sheet or explore additional protocols below.

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79040
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English
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79040
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English
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79040
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English
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Product Name
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79040
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English
Document Type
Product Name
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79040
Lot #
All
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English
Document Type
Product Name
Catalog #
79040
Lot #
All
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English
Document Type
Product Name
Catalog #
79040
Lot #
All
Language
English
Document Type
Product Name
Catalog #
79040
Lot #
All
Language
English
Document Type
Product Name
Catalog #
79040
Lot #
All
Language
English
Document Type
Product Name
Catalog #
79040
Lot #
All
Language
English

Resources and Publications

Publications (1)

SPP1 + macrophages cause exhaustion of tumor-specific T cells in liver metastases R. Trehan et al. Nature Communications 2025 May

Abstract

Functional tumor-specific CD8+ T cells are essential for effective anti-tumor immune response and immune checkpoint inhibitor therapy. Here we show that, compared to other organ sites, primary, metastatic liver tumors in murine models contain a higher number of tumor-specific CD8+ T cells which are also dysfunctional. High-dimensional, multi-omic analysis of patient samples reveals a higher frequency of exhausted tumor-reactive CD8+ T cells and enriched interactions between these cells and SPP1+ macrophages in profibrotic, alpha-SMA rich regions specifically in the liver. Differential pseudotime trajectory inference analysis reveals that extrahepatic signaling promotes an intermediate cell (IC) population in the liver, characterized by co-expression of VISG4, CSF1R, CD163, TGF-βR, IL-6R, and SPP1. Analysis of premetastatic adenocarcinoma patient samples reveals enrichment of this population may predict liver metastasis. These findings suggest a mechanism by which extrahepatic tumors drive liver metastasis by promoting an IC population that inhibits tumor-reactive CD8+ T cell function. SPP1+ macrophages and CD8 + exhausted T cells are known to crosstalk. Here, the authors discover that extrahepatic tumors facilitate liver metastasis by promoting the formation of an intermediate macrophage population in the liver that inhibits tumor-reactive CD8+ T cell function.