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    What Makes Plasmids Special?

    Plasmids have specific elements that make them powerful genetic tools:

    • Origin of Replication (ORI): A DNA sequence that allows plasmids to replicate independently in host cells. This ensures plasmid duplication during cell division.

    • Selectable Marker: Often an antibiotic resistance gene that helps identify cells containing the plasmid. Cells that successfully take up the plasmid survive when exposed to the antibiotic.

    • Multiple Cloning Site (MCS): A short sequence containing recognition sites for multiple restriction enzymes, allowing insertion of foreign DNA. In expression plasmids, the MCS is placed near a promoter for controlled gene expression.

    • Insert or Gene of Interest (GOI): The DNA fragment inserted into the plasmid for study or expression, which could be a coding gene, regulatory element, or functional DNA sequence.

    Feature

    Chromosomal DNA

    Plasmid DNA

    Extraction Focus

    Isolates the entire genome for comprehensive analysis

    Specifically isolates small, circular DNA molecules

    Purpose

    Obtain complete genomic material

    Extract plasmid DNA for genetic engineering and cloning

    Yield & Quality

    Generally higher

    Lower but optimized for cloning applications

    Method

    Breaks down the cell wall and lyses the plasma membrane

    Uses controlled alkaline lysis and neutralization to recover plasmids

    Applications

    Genotyping, sequencing, gene expression analysis

    Cloning, transformation, studying gene function, protein production

    Replication

    Requires host machinery

    Self-replicating in host cells

    Plasmid Cloning and Transformation

    Plasmid cloning and transformation are essential techniques in molecular biology that allow scientists to insert specific genes into bacterial cells for replication and study.

    Why Use Plasmid Cloning?

    • To produce specific proteins, such as recombinant insulin or GFP (green fluorescent protein).

    • To study gene function by modifying or inserting new sequences.

    • To engineer bacteria or cells for synthetic biology and genetic research.

    The DNA Cloning Process: A Step-by-Step Guide

    1. Isolating the Gene – Scientists extract or synthesize the target gene using PCR or restriction enzymes.

    2. Preparing the Plasmid – The plasmid vector is cut with specific restriction enzymes to create compatible ends.

    3. Inserting the Gene – The target gene is joined with the plasmid using DNA ligase, forming a recombinant plasmid.

    4. Transforming Bacteria – The recombinant plasmid is introduced into E. coli using heat shock or electroporation, allowing bacteria to take up the plasmid and replicate it.

    Common Cloning Vectors: pBR322 vs. pUC18

    pBR322 Plasmid (4,363 bp) (Cat# 04821225)

    • Antibiotic Resistance: Ampicillin (AmpR) and tetracycline (TetR) genes allow for selection.

    • Multiple Restriction Sites: Enzymes like PstI (AmpR) and BamHI, SalI (TetR) enable insert screening by disrupting antibiotic resistance.

    • Moderate Copy Number (~15-20 copies per cell): Useful for controlled gene expression.

    pUC18 Plasmid (2,686 bp) (Cat# 04821226)

    • High Copy Number (~500-700 copies per cell): Allows for a higher plasmid yield.

    • Antibiotic Resistance: Ampicillin (AmpR) for selection.

    • MCS in lacZα Gene: Enables blue-white screening, where successful cloning disrupts the lacZ gene, preventing blue color formation.

    Transformation Process: Introducing Plasmids into Bacteria

    Once the plasmid is ready, it must be introduced into bacterial cells for replication.

    Two Common Methods:

    • Heat Shock Transformation: Rapid temperature change helps bacterial cells take up plasmids.

    • Electroporation: Uses an electrical pulse to create temporary pores in bacterial membranes, increasing transformation efficiency.

    Media for Bacterial Growth

    After transformation, bacteria must grow in a nutrient-rich environment:

    Selection and Screening

    • Antibiotic Selection: Only transformed bacteria survive on plates with antibiotics (e.g., ampicillin, kanamycin).

    Antibiotics

    SKU

    Actinomycin D

    0219603505

    Alamethicin

    0215900905

    Amikacin

    02150342

    Amphotericin-B

    0916723

    Ampicillin (gamma irradiated), molecular biology grade

    0219419920

    Aztreonam

    02150415

    Blasticidin S hydrochloride

    02150477

    Carbenicillin Disodium Salt

    02195092

    Cefotaxime, sodium salt

    02154947

    Chloramphenicol

    02190321

    Ciprofloxacin hydrochloride

    02180935

    G418 disulfate

    02158782

    G418 Sulfate Solution

    0916725

    Gentamicin sulfate

    0916760

    Gentamycin sulfate

    02194530

    Hygromycin B

    02194170

    Kanamycin

    091672048

    Kanamycin sulfate

    02194531

    Neomycin sulfate

    02194533

    Oxytetracycline hydrochloride

    0215014510

    Paromomycin sulfate

    02194535

    Penicillin G Sodium Salt

    02194537

    Penicillin-Streptomycin

    0916704

    Pen-strep-amphotericin

    091674049

    • Screening Techniques:

      • Blue-White Screening – Used for vectors with lacZα. Successful recombinants appear white, while non-recombinants stay blue.

      • Colony PCR or Restriction Digestion – Confirms if the correct insert is present.

    Plasmid DNA Extraction: Miniprep vs. Midiprep?

    SPINeasy® Plasmid Miniprep Kit (Cat#116534050)

    • Purpose: Extracts up to 20 µg of plasmid DNA from bacteria.

    • Technology: Silica-membrane spin-column for fast DNA purification.

    • Processing Time: ~25 minutes.

    • Sample Size: 1 – 5 mL bacterial culture.

    • Elution Volume: 50 μL.

    SPINeasy® Plasmid Midiprep Kit (Cat#116539025)

    • Purpose: Extracts up to 1 mg of plasmid DNA for larger-scale applications.

    • Technology: Silica-membrane spin-column for higher yields.

    • Processing Time: Rapid purification in a simple workflow.

    • Sample Size: 25 – 50 mL bacterial culture.

    • Elution Volume: 500 μL.

    Verifying Your Cloned Plasmids

    Once you’ve cloned a plasmid, you must check if it contains the correct insert.

    Common Verification Methods:

    • Gel Electrophoresis: Confirms plasmid size and integrity.

    • Restriction Digestion: Cutting the plasmid with restriction enzymes reveals expected fragment sizes.

    • Sanger Sequencing: Provides precise confirmation of the inserted sequence.

    ✅ Tip: If your gel shows unexpected band patterns, your plasmid may have relegated incorrectly!

    Conclusion

    Understanding plasmids and their role in genetic engineering is essential for cloning experiments. Whether you’re starting your first transformation or optimizing your plasmid extraction, having the right tools makes all the difference.

     

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