Restriction Enzymes RsaI / AfaI

A restriction enzyme or restriction endonuclease is defined as a protein that recognizes a specific, short nucleotide sequence and cuts the DNA only at or near that site, known as restriction site or target sequence. The four most common types of restriction enzymes include: Type I (cleaves at sites remote from a recognition site), Type II (cleaves within or at short specific distances from a recognition site), Type III (cleave at sites a short distance from a recognition site), and Type IV (targets modified DNA- methylated, hydroxymethylated and glucosyl-hydroxymethylated DNA). The most common challenges with restriction digest include- 1. inactivation of the enzyme, 2. incomplete or no digestion, and 3. unexpected cleavage. The enzyme should always be stored at -20C and multiple freeze-thaw cycles should be avoided in order to maintain optimal activity. Always use a control DNA digestion with the enzyme to ensure adequate activity (to avoid interference due to high glycerol in the enzyme). For complete digestion, make sure that the enzyme volume is 1/10th of the total reaction volume, the optimal temperature is constantly maintained throughout the reaction, the total reaction time is appropriately calculated based on the amount of DNA to be digested, appropriate buffers should be used to ensure maximal enzymatic activity, and in case of a double digest, make sure that the two restriction sites are far enough so that the activity of one enzyme cannot interfere with the activity of the other. Star activity (or off-target cleavage) and incomplete cleavage are potential challenges which may occur due to suboptimal enzymatic conditions or inappropriate enzyme storage. To avoid these, follow the recommended guidelines for storage and reactions, and always check for the efficacy of digestion along with purification of digested products on an agarose gel.

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RsaI NEB#R0167

New England BioLabs

Upstream tips	Protocol tips	Downstream tips
	Prior to the RFLP, the multiplex PCR product was separated into three tubes for the genotyping of CYP3A44, CYP3A418B and CYP3A4*22 using BsmAI (NEB® Inc, Massachusetts, USA), RsaI (NEB® Inc, Massachusetts, USA) and BseYI (NEB® Inc, Massachusetts, USA) restriction enzymes (RE), respectively. The first tube contained 2.0 U BsmAI, 1× CutSmart NEBuffer® (NEB® Inc, Massachusetts, USA), 0.3–0.4 μg of PCR products and 9.2 μL doubly distilled water followed by incubation at 55 °C for 60 min. (Alpha Innotech, USA). The second tube contained 4.0 U of RsaI, 1× CutSmart NEBuffer® (NEB® Inc, Massachusetts, USA), 0.3–0.4 μg fresh PCR products and 8.8 doubly distilled water, followed by incubation at 37 °C for 60 min. The third tube contained 6.0 U BseYI, 1× NEBuffer 3.1® (NEB® Inc, Massachusetts, USA), 0.3–0.4 μg fresh PCR template and 8.4 μL doubly distilled water; incubated at 37 °C for 60 min followed by an inactivation step at 80 °C for 20 min. The incubation for all RFLP samples was carried out using an Accublock Digital Dry Bath.

Protocol tips
Prior to the RFLP, the multiplex PCR product was separated into three tubes for the genotyping of CYP3A44, CYP3A418B and CYP3A4*22 using BsmAI (NEB® Inc, Massachusetts, USA), RsaI (NEB® Inc, Massachusetts, USA) and BseYI (NEB® Inc, Massachusetts, USA) restriction enzymes (RE), respectively. The first tube contained 2.0 U BsmAI, 1× CutSmart NEBuffer® (NEB® Inc, Massachusetts, USA), 0.3–0.4 μg of PCR products and 9.2 μL doubly distilled water followed by incubation at 55 °C for 60 min. (Alpha Innotech, USA). The second tube contained 4.0 U of RsaI, 1× CutSmart NEBuffer® (NEB® Inc, Massachusetts, USA), 0.3–0.4 μg fresh PCR products and 8.8 doubly distilled water, followed by incubation at 37 °C for 60 min. The third tube contained 6.0 U BseYI, 1× NEBuffer 3.1® (NEB® Inc, Massachusetts, USA), 0.3–0.4 μg fresh PCR template and 8.4 μL doubly distilled water; incubated at 37 °C for 60 min followed by an inactivation step at 80 °C for 20 min. The incubation for all RFLP samples was carried out using an Accublock Digital Dry Bath.

Protocol tips

Prior to the RFLP, the multiplex PCR product was separated into three tubes for the genotyping of CYP3A4*4, CYP3A4*18B and CYP3A4*22 using BsmAI (NEB® Inc, Massachusetts, USA), RsaI (NEB® Inc, Massachusetts, USA) and BseYI (NEB® Inc, Massachusetts, USA) restriction enzymes (RE), respectively. The first tube contained 2.0 U BsmAI, 1× CutSmart NEBuffer® (NEB® Inc, Massachusetts, USA), 0.3–0.4 μg of PCR products and 9.2 μL doubly distilled water followed by incubation at 55 °C for 60 min. (Alpha Innotech, USA). The second tube contained 4.0 U of RsaI, 1× CutSmart NEBuffer® (NEB® Inc, Massachusetts, USA), 0.3–0.4 μg fresh PCR products and 8.8 doubly distilled water, followed by incubation at 37 °C for 60 min. The third tube contained 6.0 U BseYI, 1× NEBuffer 3.1® (NEB® Inc, Massachusetts, USA), 0.3–0.4 μg fresh PCR template and 8.4 μL doubly distilled water; incubated at 37 °C for 60 min followed by an inactivation step at 80 °C for 20 min. The incubation for all RFLP samples was carried out using an Accublock Digital Dry Bath.

Publication protocol 1 Relevant paper

RsaI (10 U/µL)

Thermo Fisher Scientific

Upstream tips	Protocol tips	Downstream tips
	For 2D agarose gel analysis, 10μg DNA was digested overnight at 37°C with 10U HinfI (Thermo Fisher), 10U RsaI (Thermo Fisher) and 2μg/mL RNase A (Takara). The reaction was terminated with EDTA and analyzed by 2D agarose gel electrophoresis. 30U RecJf (New England Biolabs) was added for removing 5' single-stranded DNA. For internal gaps/nicks analysis, 5μg genomic DNA was digested overnight at 37°C with 5U HinfI (Thermo Fisher), 5U RsaI (Thermo Fisher) and 1μg/mL Ribonuclease A (RNase A, Takara) and purified with QIAquick PCR Purification kit (Qiagen).

Protocol tips
For 2D agarose gel analysis, 10μg DNA was digested overnight at 37°C with 10U HinfI (Thermo Fisher), 10U RsaI (Thermo Fisher) and 2μg/mL RNase A (Takara). The reaction was terminated with EDTA and analyzed by 2D agarose gel electrophoresis. 30U RecJf (New England Biolabs) was added for removing 5' single-stranded DNA. For internal gaps/nicks analysis, 5μg genomic DNA was digested overnight at 37°C with 5U HinfI (Thermo Fisher), 5U RsaI (Thermo Fisher) and 1μg/mL Ribonuclease A (RNase A, Takara) and purified with QIAquick PCR Purification kit (Qiagen).

Protocol tips

For 2D agarose gel analysis, 10μg DNA was digested overnight at 37°C with 10U HinfI (Thermo Fisher), 10U RsaI (Thermo Fisher) and 2μg/mL RNase A (Takara). The reaction was terminated with EDTA and analyzed by 2D agarose gel electrophoresis. 30U RecJf (New England Biolabs) was added for removing 5' single-stranded DNA.

For internal gaps/nicks analysis, 5μg genomic DNA was digested overnight at 37°C with 5U HinfI (Thermo Fisher), 5U RsaI (Thermo Fisher) and 1μg/mL Ribonuclease A (RNase A, Takara) and purified with QIAquick PCR Purification kit (Qiagen).

Manufacturer protocol Publication protocol 1 Relevant paper

AfaI (RsaI) restriction enzyme

Takara Bio Inc

Upstream tips	Protocol tips	Downstream tips
	The other three libraries were each made from DNA digested with three different restriction enzymes; AluI (Fermentas), HaeIII (TaKaRa Bio Inc.) and AfaI (TaKaRa Bio Inc.).	Each digested DNA was purified using Wizard SV Gel and PCR Clean-Up System (Promega, Madison WI, USA) and ligated with double stranded DNA linkers (linker 1: 50 -GTTTAGCCTTGTAGCAGAAGC-30 and linker 2: 50 -pGCTTCTGCTACAAGGCTAAACAAAA-30 ).

Protocol tips
The other three libraries were each made from DNA digested with three different restriction enzymes; AluI (Fermentas), HaeIII (TaKaRa Bio Inc.) and AfaI (TaKaRa Bio Inc.).
Downstream tips
Each digested DNA was purified using Wizard SV Gel and PCR Clean-Up System (Promega, Madison WI, USA) and ligated with double stranded DNA linkers (linker 1: 50 -GTTTAGCCTTGTAGCAGAAGC-30 and linker 2: 50 -pGCTTCTGCTACAAGGCTAAACAAAA-30 ).

Manufacturer protocol Publication protocol 1 Relevant paper

FastDigest RsaI

Thermo Fisher Scientific

Upstream tips	Protocol tips	Downstream tips
	Purified products were digested with restriction enzyme FastDigest RsaI (Thermo Fisher Scientific, Inc.) at 37°C for 1–2 h.	The digested products were recovered using 20 uL of sterile deionized water and ethanol precipitation.

Protocol tips
Purified products were digested with restriction enzyme FastDigest RsaI (Thermo Fisher Scientific, Inc.) at 37°C for 1–2 h.
Downstream tips
The digested products were recovered using 20 uL of sterile deionized water and ethanol precipitation.

Manufacturer protocol Publication protocol 1 Relevant paper

RsaI R6371

Promega

Upstream tips	Protocol tips	Downstream tips
	One microgram of DNA was digested for 6 h with 10 units of RsaI (Promega) in a 20-μl reaction volume. The restriction fragments were blunt-end ligated with phosphorylated EcoRI linkers (Promega), using T4 DNA ligase (Promega).

Protocol tips
One microgram of DNA was digested for 6 h with 10 units of RsaI (Promega) in a 20-μl reaction volume. The restriction fragments were blunt-end ligated with phosphorylated EcoRI linkers (Promega), using T4 DNA ligase (Promega).

Manufacturer protocol Publication protocol 1 Relevant paper

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