Serie: Chromatin-Immunpräzipitation - ChIP

Chromatin immunoprecipitation, abbreviated as ChIP, is a technique for studying the protein-DNA interactions that regulate gene expression.

In eukaryotes, DNA is wrapped around histone proteins and forms a complex known as a nucleosome, which further groups together into a structure known as chromatin to aid in the tight packaging of DNA in the cells.

Gene expression is regulated through histone modifications that uncoil or tighten these structures as well as proteins that associate with cis-regulatory regions on the DNA.

In ChIP, the chromatin is broken down and antibodies that bind to histone modifications or regulatory proteins, are used to isolate the target molecules with the associated DNA.

The first step in this process is to crosslink the protein to the DNA with the help of a crosslinking agent, such as formaldehyde. This immobilizes the protein on the DNA marking the binding site of the protein. After crosslinking, the chromatin is mechanically sheared into short fragments ranging from 100 to 200 base pairs. This process is known as X-ChIP.

An alternative method is N-ChIP, in which nucleases directly digest DNA from the chromatin into short fragments, without any prior cross-linking.

Immunoprecipitation is carried out by introducing antibodies that target the regulatory proteins in the solution containing sheared or digested DNA. These antibodies are linked to agents that help in selective isolation.

One common method is linking the antibodies to magnetic beads. A magnet is used to isolate the antibodies along with any bound molecules.

The complex is rinsed to wash off any loosely associated contaminants. The target molecules are detached with the help of a detergent, such as SDS.

In the case of X-ChiP, crosslinking is reversed with the help of elevated temperatures, and the associated regulators or histones are degraded with the help of proteases, leaving behind the DNA.

Sequencing of the associated DNA can help identify the cis-regulatory sequence that the protein of interest was bound to or the gene whose expression is modulated by a particular histone modification.

Chromatin immunoprecipitation, or ChIP, is an antibody-based technique used to identify sites on DNA that bind to transcription factors of interest or histone proteins. It also helps determine the type of histone modifications such as acetylation, phosphorylation, or methylation.

Types of ChIP

ChIP can be divided into two types - X-ChIP and N-ChIP. X-ChIP involves in vivo cross-linking of histones and regulatory proteins to DNA, fragmenting the DNA by sonication, and isolating the protein-DNA complexes by immunoprecipitating them with specific antibodies. On the other hand, N-ChIP does not involve cross-linking of DNA to proteins, and digestion is carried out using nucleases.

Downstream analysis of DNA - protein interactions

After isolating the DNA of interest, techniques such as PCR, microarrays, or southern blot can be used for analysis. Alternatively, this DNA can be used for deep sequencing, known as ChIP-Seq. ChIP can be modified using other methodologies for different analysis such as ChIA-PET, a technique that combines the principles of ChIP with chromosome conformation capture to detect long-range chromatin interactions mediated via a protein of interest; enChIP, a technique which employs the CRISPR/Cas9 system to target specific genomic regions and RIP-ChIP/RIP-Seq, a modification of ChIP used to analyze protein-RNA interactions.

Comparison between N-ChIP and X-ChIP

N-ChIP and X-ChIP have their own advantages and disadvantages. N-ChIP results in stronger antibody binding and efficient and highly specific immuno-precipitation. However, N-ChIP is suitable only in the case of tightly bound proteins such as histones, as transcription factors may get detached during processing. Additionally, not all of the nuclease-digested chromatin gets solubilized, resulting in the missing out of certain fractions of the sample. X-ChIP is an excellent methodology for studying transcription factors that are not bound tightly to the DNA due to its cross-linking step. X-ChIP assay is also more sensitive than N-ChIP and requires lower amounts of samples as well as antibodies. Disadvantages of X-chip include possible difficulty in fragmentation due to excess cross-linking and false positives due to the cross-linking of transient-DNA protein interactions.

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