AM1921
Invitrogen™ PARIS™ Kit
Manufacturer: Invitrogen™
Select a Size
| Pack Size | SKU | Availability | Price |
|---|---|---|---|
| Each of 1 | AM1921-Each-of-1 | In Stock | ₹ 48,760.00 |
AM1921 - Each of 1
In Stock
Quantity
1
Base Price: ₹ 48,760.00
GST (18%): ₹ 8,776.80
Total Price: ₹ 57,536.80
Content And Storage
• 30 mL Cell Disruption Buffer; 4°C• 25 mL Cell Fractionation Buffer; 4°C• 30 mL 2X Lysis/Binding Solution; 4°C• 40 mL Wash Solution 1; 4°C• 80 mL Wash Solution 2/3 Concentrate; 4°C• 4 mL Lithium Chloride Precipitation Solution; 4°C• 50 Filter Cartridges; room temperature• 100 Collection Tubes; room temperature• 10 mL Elution Solution; room temperature
Purification Time
20 min.
Sample Type
Cells, Tissue
High-throughput Compatibility
Not High-throughput Compatible (Manual)
Quantity
50 Preps
Starting Material Amount
Cells: ≤107cellsTissue: ≤75 mg tissue
Isolation Technology
Spin Column (Glass Fiber Filter)
Elution Volume
50 to 200 μL
Final Product Type
Total RNA and Protein
For Use With (Application)
RT-PCR, qPCR, cDNA library construction, NGS, microarray analysis, blot hybridization, Northern/Western blotting, in vitro translation, nuclease protection assays, nucleic acid labeling, enzymatic assays, immunoprecipitation, gel shift assays, 2D gel electrophoresis
Shipping Condition
Room Temperature
Yield
≤1 μg per 105cells≤10 μg per 1 mg tissue
Related Products
Description
- Description The Invitrogen™ PARIS™ system is for the isolation of both RNA and native protein from the same experimental sample
- The kit also permits separation of nuclear and cytoplasmic fractions prior to RNA and/or protein isolation
- The kit contains sufficient reagents for 50 purifications from1 to 75 mg of tissue or 100 to 10 7 cells each
- • Fast, simple procedure • Isolate nuclear and cytoplasmic RNA and protein from cultured cells • Isolate total RNA and protein from cultured cells or tissues • No phenol extraction or alcohol precipitation • Reduces time, cost, and variability between independent experimental samples Isolation of high-quality RNA is the first step for a variety of gene expression analyses
- Very often, complementary studies at the protein level are also required
- Usually these analyses are performed using different aliquots of the same experimental sample
- However, when working with rare, difficult to obtain, or very small samples, it is sometimes impractical to isolate RNA and native proteins independently
- In studies involving large numbers of samples, expensive reagents, or inherent variability (e.g., cell transfection), the addition of independent experimental samples is not only costly and time consuming, but may also lead to inconsistent results
- To solve these issues, the Protein And RNA Isolation System (PARIS™ system) has been developed
- It allows for the isolation of both RNA and protein from the same experimental sample (see Figure)
- Using the PARIS™ system, RNA and protein can be isolated simultaneously from whole cell lysates
- Alternatively, RNA and protein can be isolated from separate nuclear and cytoplasmic fractions
- Tissue or cultured cells are first homogenized in ice-cold Cell Disruption Buffer to prepare a total cell lysate
- Since the homogenization is performed quickly on ice and in the presence of detergent, both protein and RNA can be purified directly from this lysate
- For RNA isolation, a part of the total cell lysate is immediately mixed with an equal volume of Lysis/Binding Solution
- Total RNA is then purified from the mixture using an RNA binding glass fiber filter
- After three rapid washing steps, high-quality RNA is eluted in a concentrated form
- The entire procedure can be completed in less than 20 minutes
- Note: This kit is not recommended for tissues with high levels of ribonucleases, such as pancreas
- Compatible with Most Downstream Applications The RNA isolated from total, nuclear, or cytoplasmic fractions with the PARIS™ procedure can be used in a variety of downstream applications, including blot hybridization, in vitro translation, cDNA synthesis, and RT-PCR
- A DNase I treatment is recommended for RNA that will be used for RT-PCR experiments (see Accessory Products)
- Protein fractions can be used directly for most common applications, including functional assays, immunoprecipitation, western blotting, or two-dimensional gel electrophoresis (see Figures)
- Accessory Products: TURBO™ DNA- free ™ or DNA- free ™ DNase Treatment and Removal Reagents (Cat
- No. AM1907 and AM1906, respectively) are ideal to quickly remove trace amounts of DNA from the total and nuclear RNA samples without phenol extraction or alcohol precipitation
- The cytoplasmic RNA fraction is virtually free of DNA contamination
- Order Info Shipping Condition: Room temperature
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Content And Storage: • 30 mL Cell Disruption Buffer; 4°C• 25 mL Cell Fractionation Buffer; 4°C• 30 mL 2X Lysis/Binding Solution; 4°C• 40 mL Wash Solution 1; 4°C• 80 mL Wash Solution 2/3 Concentrate; 4°C• 4 mL Lithium Chloride Precipitation Solution; 4°C• 50 Filter Cartridges; room temperature• 100 Collection Tubes; room temperature• 10 mL Elution Solution; room temperature
Purification Time: 20 min.
Sample Type: Cells, Tissue
High-throughput Compatibility: Not High-throughput Compatible (Manual)
Quantity: 50 Preps
Starting Material Amount: Cells: ≤107cellsTissue: ≤75 mg tissue
Isolation Technology: Spin Column (Glass Fiber Filter)
Elution Volume: 50 to 200 μL
Final Product Type: Total RNA and Protein
For Use With (Application): RT-PCR, qPCR, cDNA library construction, NGS, microarray analysis, blot hybridization, Northern/Western blotting, in vitro translation, nuclease protection assays, nucleic acid labeling, enzymatic assays, immunoprecipitation, gel shift assays, 2D gel electrophoresis
Shipping Condition: Room Temperature
Yield: ≤1 μg per 105cells≤10 μg per 1 mg tissue
Content And Storage:
• 30 mL Cell Disruption Buffer; 4°C• 25 mL Cell Fractionation Buffer; 4°C• 30 mL 2X Lysis/Binding Solution; 4°C• 40 mL Wash Solution 1; 4°C• 80 mL Wash Solution 2/3 Concentrate; 4°C• 4 mL Lithium Chloride Precipitation Solution; 4°C• 50 Filter Cartridges; room temperature• 100 Collection Tubes; room temperature• 10 mL Elution Solution; room temperature
Purification Time:
20 min.
Sample Type:
Cells, Tissue
High-throughput Compatibility:
Not High-throughput Compatible (Manual)
Quantity:
50 Preps
Starting Material Amount:
Cells: ≤107cellsTissue: ≤75 mg tissue
Isolation Technology:
Spin Column (Glass Fiber Filter)
Elution Volume:
50 to 200 μL
Final Product Type:
Total RNA and Protein
For Use With (Application):
RT-PCR, qPCR, cDNA library construction, NGS, microarray analysis, blot hybridization, Northern/Western blotting, in vitro translation, nuclease protection assays, nucleic acid labeling, enzymatic assays, immunoprecipitation, gel shift assays, 2D gel electrophoresis
Shipping Condition:
Room Temperature
Yield:
≤1 μg per 105cells≤10 μg per 1 mg tissue
Content And Storage: Store Nuclease-free Water, Microfuge Tubes and Microfuge tubes with Spin Columns at room temperature. Store 2X Binding Solution, Wash Solution 1, Wash Solution 2 and Oligo(dT) Cellulose at 4°C. Store RNA Storage Solution, 5M Ammonium Acetate and Glycogen(5 mg/mL) at -20°C.
Purification Time: __
Sample Type: Total RNA
High-throughput Compatibility: Not High-throughput Compatible (Manual)
Quantity: __
Starting Material Amount: __
Isolation Technology: Magnetic Bead, Oligo dT Affinity
Elution Volume: __
Final Product Type: mRNA
For Use With (Application): Microarray Analysis, Reverse Transcriptase PCR (RT-PCR), Microinjection, Nucleic Acid Labeling, In Vitro Translation, cDNA Library Construction, Northern Blotting, Nuclease Protection Assays
Shipping Condition: Room Temperature
Yield: __
Content And Storage:
Store Nuclease-free Water, Microfuge Tubes and Microfuge tubes with Spin Columns at room temperature. Store 2X Binding Solution, Wash Solution 1, Wash Solution 2 and Oligo(dT) Cellulose at 4°C. Store RNA Storage Solution, 5M Ammonium Acetate and Glycogen(5 mg/mL) at -20°C.
Purification Time:
__
Sample Type:
Total RNA
High-throughput Compatibility:
Not High-throughput Compatible (Manual)
Quantity:
__
Starting Material Amount:
__
Isolation Technology:
Magnetic Bead, Oligo dT Affinity
Elution Volume:
__
Final Product Type:
mRNA
For Use With (Application):
Microarray Analysis, Reverse Transcriptase PCR (RT-PCR), Microinjection, Nucleic Acid Labeling, In Vitro Translation, cDNA Library Construction, Northern Blotting, Nuclease Protection Assays
Shipping Condition:
Room Temperature
Yield:
__
Content And Storage: Store Nuclease-free Water, Microfuge Tubes and Microfuge tubes with Spin Columns at room temperature. Store 2X Binding Solution, Wash Solution 1, Wash Solution 2 and Oligo(dT) Cellulose at 4°C. Store RNA Storage Solution, 5M Ammonium Acetate and Glycogen(5 mg/mL) at -20°C.
Purification Time: __
Sample Type: RNA
High-throughput Compatibility: Not High-throughput Compatible (Manual)
Quantity: __
Starting Material Amount: __
Isolation Technology: Magnetic Bead, Oligo dT Affinity
Elution Volume: __
Final Product Type: mRNA
For Use With (Application): Microarray Analysis, Reverse Transcriptase PCR (RT-PCR), Microinjection, Nucleic Acid Labeling, In Vitro Translation, cDNA Library Construction, Northern Blotting, Nuclease Protection Assays
Shipping Condition: __
Yield: __
Content And Storage:
Store Nuclease-free Water, Microfuge Tubes and Microfuge tubes with Spin Columns at room temperature. Store 2X Binding Solution, Wash Solution 1, Wash Solution 2 and Oligo(dT) Cellulose at 4°C. Store RNA Storage Solution, 5M Ammonium Acetate and Glycogen(5 mg/mL) at -20°C.
Purification Time:
__
Sample Type:
RNA
High-throughput Compatibility:
Not High-throughput Compatible (Manual)
Quantity:
__
Starting Material Amount:
__
Isolation Technology:
Magnetic Bead, Oligo dT Affinity
Elution Volume:
__
Final Product Type:
mRNA
For Use With (Application):
Microarray Analysis, Reverse Transcriptase PCR (RT-PCR), Microinjection, Nucleic Acid Labeling, In Vitro Translation, cDNA Library Construction, Northern Blotting, Nuclease Protection Assays
Shipping Condition:
__
Yield:
__
Content And Storage: Store 1X PBS pH 7.4, RNAlater;™ Solution, Rubber Septum Cap, White Slip Connector, Transfer Spike, LeukoLOCK™ Filter, Elution Solution, LeukoLOCK™ Lysis/Binding Solution, LeukoLOCK™ pH Adjustment Solution, Processing Tubes, Wash Solution 1 Concentrate, Wash Solution 2/3 Concentrate and Nuclease-Free Water at room temperature.Store RNA Binding Beads at 4°C.Store 1X LeukoLOCK™ DNase Buffer, Proteinase K, and TURBO™ DNase at -20°C.
Purification Time: __
Sample Type: Cells, Blood
High-throughput Compatibility: Not High-throughput Compatible (Manual)
Quantity: 20 preps
Starting Material Amount: Up to 10 ml whole blood
Isolation Technology: Leukocyte Capture Filter, Magnetic Bead
Elution Volume: __
Final Product Type: Total RNA
For Use With (Application): Microarray Analysis, Real-Time Quantitative PCR (qPCR), Reverse Transcriptase PCR (RT-PCR), Nuclease Protection Assays, Northern Blotting, cDNA Library Construction
Shipping Condition: __
Yield: __
Content And Storage:
Store 1X PBS pH 7.4, RNAlater;™ Solution, Rubber Septum Cap, White Slip Connector, Transfer Spike, LeukoLOCK™ Filter, Elution Solution, LeukoLOCK™ Lysis/Binding Solution, LeukoLOCK™ pH Adjustment Solution, Processing Tubes, Wash Solution 1 Concentrate, Wash Solution 2/3 Concentrate and Nuclease-Free Water at room temperature.Store RNA Binding Beads at 4°C.Store 1X LeukoLOCK™ DNase Buffer, Proteinase K, and TURBO™ DNase at -20°C.
Purification Time:
__
Sample Type:
Cells, Blood
High-throughput Compatibility:
Not High-throughput Compatible (Manual)
Quantity:
20 preps
Starting Material Amount:
Up to 10 ml whole blood
Isolation Technology:
Leukocyte Capture Filter, Magnetic Bead
Elution Volume:
__
Final Product Type:
Total RNA
For Use With (Application):
Microarray Analysis, Real-Time Quantitative PCR (qPCR), Reverse Transcriptase PCR (RT-PCR), Nuclease Protection Assays, Northern Blotting, cDNA Library Construction
Shipping Condition:
__
Yield:
__