Although the vials are bottled using aseptic techniques, heat-treated vials, and sterile stock solutions, they are not considered or guaranteed to be sterile. If sterile material is needed for an experiment, the material can be filtered through a 0.2 micron filter designed for use with biological fluids.
The Reconstitution Buffers, Catalog #s RB01 through RB07, are RUO (Research Use Only) products and are not guaranteed to be sterile. As part of Quality Control process prior to release, Reconstitution Buffers RB01 through RB07 undergo testing including a 7 day microbial Bioburden test, as well as a test for Endotoxin via LAL method (specification of < 0.25 EU/mL). If sterile buffer is required, it is recommended the buffer can be filtered through a 0.2 micron filter designed for use with biological fluids
The enzyme would remain active for a limited amount of time, but we do not have data to suggest how long the activated enzyme will retain activity. We recommend activating the enzyme and using immediately for each experiment.
The bioassay listed on the protein datasheets describes the method R&D Systems uses to QC the protein. There are many other potential ways to use each protein. We maintain a database of references citing the use of products in other applications or with different cell types. Please click the Citations tab on the product-specific web page or contact Technical Service for more information.
Our proteins and antibodies can be used for in vivo experiments in animals in approved studies, but not in humans or veterinary animals. R&D Systems does not perform any in vivo testing. Therefore, the activity and half-life in these applications are uncertain. References for in vivo use may be found by clicking on the "Citations" tab on the product specific web page. We recommend using the carrier-free forms of proteins for in vivo experiments and Technical Service can provide lot-specifc endotoxin levels upon request.
It is our policy not to assign CAS numbers to our recombinant proteins or antibodies unless there is a hazard which needs to be disclosed. While of high purity, they are still considered biological mixtures, and not pure synthesized chemicals.
R&D Systems offers an expanding line of biotinylated proteins, with more information found on the following link: https://www.rndsystems.com/products/active-biotinylated-proteins. Products can also be easily identified on the Product Search Page (https://www.rndsystems.com/products), and filtering for Conjugate on Biotin.Please inquire if you are unable to find your protein of interest.
R&D Systems intentionally sells most proteins by mass rather than units. To follow an assay protocol given in units, or to compare a commercially available product sold on a unit basis, one must verify how the unit was defined. It is strongly recommended that a dose response be performed when beginning experiments, or with new lots or vendors. Our recommendation is using the midpoint of our ED50 range as the midpoint in the titration, and also running samples at 5, 10, 20, or 50 fold increments above and below this point. If the author/vendor has compared their "unit" to a WHO standard unit, you may find information contained in the WHO Conversion Table on our website (https://www.rndsystems.com/resources/technical-information/unit-conversion-table) to determine roughly where to start. This table contains approximate mass to unit conversion factors based on our historical testing against WHO standards. Please note this information is for reference purposes only, and is not routinely tested for our RUO grade proteins. The WHO standards are available from the NIBSC for purchase and can be used side-by-side in your own assay to determine specific activity in units. Alternatively, please also consider our preclinical animal-free (AFL) grade or GMP grade versions which, in addition to ED50, have minimum specific activity specifications and each bottled lot is tested against the WHO standard, with specific activity reported on the lot-specific CoA.
R&D Systems lists the molecular weight of our proteins in kDa on the datasheets. The approximate conversion to molar mass is 1 Dalton = 1 gram/mol. For instance, an 8 kDa protein would be 8000 grams/mol.
The product is shipped at ambient temperature by design and will not be compromised. Lyophilization increases product stability, while reducing packing materials and shipping expense. We have performed “stress tests” on our lyophilized products. These products are subjected to 37º C for 3 days in a humidified chamber and found to be stable. These data demonstrate that lyophilized products shipped ambient and received with in a 3 day window retain full activity. We will guarantee and support the product performance when delivered and properly stored within this timeframe. If the product was not delivered within 3 days to your facility or was not stored properly upon receipt, please contact Technical Service.
There are multiple reasons why you may not observe a lyophilized pellet in your vial. The three most common reasons for this observation are: (1) The lyophilized product has become dislodged from the bottom of the vial during shipping/handling and is dispersed on the vial wall or cap. Tapping the vial firmly on the bench or a quick spin in a centrifuge may bring the lyophilized product back to the bottom of the vial. (2) When our products are bottled with a carrier protein (BSA), this protein is provided as 50 µg of carrier for every 1 µg of product which makes the resulting pellet very pronounced. Conversely, when products are offered carrier-free the pellet can be very hard to visualize or appear as a transparent film-like appearance due to this lack of carrier. (3) If the product is originally lyophilized from a solvent such as acetonitrile or ethanol and supplied carrier-free, you may not be able to visualize the pellet with the naked eye. This is a common observation does not mean the vial is empty. We would recommend tapping or centrifuging the vial to bring all the material down to the bottom of the vial, and reconstituting the product as directed on the Certificate of Analysis or datasheet. If you experience any difficulties with the product, please contact our Technical Support for assistance.
No, an Fc chimera is a recombinant protein, not an antibody. A recombinant protein may be fused to the Fc region of IgG for multiple reasons. It can be used for purification, for detecting the protein with an anti-IgG antibody in a binding assay, or to encourage the formation of disulfide-linked homodimers which increases the bioactivity of some recombinant proteins.
Yes, we recommend the carrier free protein without the BSA for this purpose. The presence of 50 μg of BSA to 1 μg of recombinant protein may affect the migration of the recombinant protein in SDS PAGE and may also mask recombinant protein bands on a membrane pre-stained with a protein visualization dye such as Ponceau S. Keep in mind that due to the expression system used and the addition of tags or other modifications to the recombinant protein, it may not migrate at the predicted molecular weight of the native molecule in natural samples.
For optimal stability and performance, we recommend storing the reconstituted protein at the reconstitution concentration in single-use aliquots of a volume no less than 20 microliters. The reconstitution conditions specified for each protein are based on in-house stability testing.
For optimal performance, enzymes should be stored at the original stock concentration and storage temperature as directed on the Certificate of Analysis or product datasheet. Individual single-use aliquots can be prepared, preferably no less than 10 uL in volume, and stored in polypropylene or siliconized tubes.
To investigate whether this is possible, please contact Technical Service (techsupport@bio-techne.com) or Custom Services (https://www.rndsystems.com/services).
E. coli-derived proteins are not glycosylated. Sf 21 and Sf 9 cells are able to partially glycosylate proteins on N-linked sites with 3-9 mannose residues. They do not incorporate galactose or sialic acid, so there is no branching of sugars. Glycosylation on O-linked sites in proteins derived from Sf 21 and Sf 9 cells is sporadic. NS0, CHO, and HEK293 cells are capable of fully glycosylating N-linked and O-linked glycosylation sites with branching sugars.
The fluorescent standard should be diluted in assay buffer and run in duplicate, reserving wells for assay buffer only to serve as blanks. Wells in the standard curve will only contain the calibration standard diluted in assay buffer. After subtracting the blank RFU, the resulting RFU versus concentration can be plotted to determine RFU/pmol. This slope (RFU/pmol) can then be inverted (pmol/RFU) and used in specific activity calculations.
R&D Systems uses a Probumin® Media Grade BSA (Millipore; Catalog # 81-068) for protein reconstitution. It is recommended that customers use the same or equivalent.
Environmental stewardship is important to R&D Systems and its employees. R&D Systems is ISO 14001:2015 Certified and as part of this we are continuously reviewing our sustainability practices and "green" options. First and foremost, the energy expended to ship back the styrofoam box is more detrimental to the environment than having the facility re-use or recycle it. Our stance is to encourage our customers to implement a recycling program locally. At R&D Systems we have chosen to reduce the use of styrofoam as much as possible by: doing extensive stability testing in order to determine which products can be shipped with minimal packaging at ambient temperatures, converting the use of non-recyclable packaging materials to recyclable plastics, cardboard, or biodegradable materials, and continuing to investigate alternatives to dry ice shipments, the use of re-usable containers, and gel packs that allow for smaller styrofoam containers. Employees were key to initiating a recycling program at our facilities. Internally, we recycle paper, plastic, cardboard, aluminum, and glass.
For sugar- and amine-labeled biotinylated proteins, multiple biotin molecules are conjugated to the protein after purification. The result is a biotinylated protein with a high biotin-to-protein ratio. This make these particular biotinylated proteins good candidates for applications that require high signal, such as flow cytometry, ELISA, SPR, and immunoprecipitation. While sugar and amine biotinylation can produce varying results (as the biotins are conjugated at potentially any free sugar or amine on the protein), Avi-tag biotinylated proteins feature biotinylation at a single site contained within the Avi-tag, a unique 15 amino acid peptide. The DNA sequence coding for the Avi-tag is inserted during cloning and contained in the final expression vector construct. Biotinylation of the Avi-tag is enzymatically performed by the E. coli biotin ligase BirA. Additionally, the consistent labeling enables uniform orientation of the protein when bound to a streptavidin-coated surface. For more information, please see https://www.rndsystems.com/products/active-biotinylated-proteins.
R&D Systems has established a policy of not limiting the useful life of a product by providing an expiration date or manufacture date for our protein and antibody products. Under proper storage conditions, proteins and antibodies tend to be stable for many years. These conditions include storing proteins as lyophilized powder, storing the product frozen (-20° C or -80° C) at protein concentrations of greater than 0.1 mg/mL, and limiting the number of freeze/thaw cycles. Please see individual product datasheets for specific instructions. Routine quality control testing by our company ensures that all products have acceptable biological activities at the time of sale. R&D Systems cannot control storage conditions of a product upon receipt by the end user. In lieu of an expiration date, we choose to offer a warranty on our protein and antibody products. All products supplied by R&D Systems are warranted to meet or exceed our published specification when used under normal conditions in your laboratory.Typically, this warranty will extend 6-12 months from time of purchase. Please see individual datasheets for specific stability claims. If the product fails during the stated period, a replacement product or credit will be issued. For details regarding our warranty please see //www.rndsystems.com/customer_service_legal.aspx.
Unless more specific directions are on the Certificate of Analysis provided with the product, we suggest the following procedure to ensure optimal recovery:1. Allow the product to be reconstituted and the reconstitution diluent to reach room temperature.2. Tap or briefly centrifuge the product vial before opening to dislodge any lyophilized material that may be dispersed on the wall or cap of the vial.3. Use the diluent and stock concentration recommended in the product datasheet. If preparing a stock concentration higher than recommended, contact Technical Service.4. After adding the diluent, re-cap the vial and invert gently by hand or place on a slow rocking platform to allow the reconstitution diluent to coat all the surfaces inside the vial.Note: Do not mix by vortexing or by pipetting the material up and down.5. Allow the vial to sit at room temperature with gentle agitation for at least 15 minutes before aliquotting or using.6. Store the reconstituted material in single use aliquots in polypropylene or siliconized tubes. Aliquots of 10 μL or larger are recommended.If the vial exhibits flakes or particulates, mix the product for a couple of hours at room temperature and then at 4 °C overnight. Please contact Technical Service at techsupport@bio-techne.com if the product does not go into solution.
While reading every 30 seconds should theoretically allow for detection of a linear trend, changing the reading frequency to every 10 or 15 seconds may better encapsulate the curve. The reading frequency may need to be optimized for best results, especially if you are using a 384-well plate.
The product datasheet and Certificates of Analysis for lyophilized proteins and antibodies will indicate the recommended reconstitution concentration. Concentration = mass/volume. Calculate the target volume by dividing mass by concentration after making certain the mass units match. For example, a 100 μg vial of an antibody may need to be reconstituted at 0.5 mg/mL. 0.5 mg/mL = 500 μg/mL. 100 μg / (500 μg/1 mL) = 0.2 mL, so 0.2 mL (200 μL) of volume would be needed for reconstitution at this concentration. Alternatively, use the Molarity and Reconstitution Calculators found under the Resources tab on R&D Systems' website.
CF stands for "carrier free." Typically our recombinant proteins are bottled with 50 μg of BSA (carrier protein) per 1 μg of proteinin order to enhance stability. The carrier-free version does not contain BSA. Usually proteins with BSA can be stored at a more dilute concentration than the carrier-free counterpart, and they may have a longer shelf-life. Generally one will want to purchase the version with BSA when adding the proteins to culture medium or for ELISA standards. Some situations where carrier-free proteins might be used would be in in vivo applications, when labeling proteins, or for other applications where the BSA might interfere with the experiment.
BSA as a carrier can enhance the stability of a given protein or permit storage at lower concentrations for a great length of time. For certain applications, however, BSA can be problematic. It would not be necessary to add BSA upon reconstitution unless required for your specific application. Please refer to the lot-specific Certificate of Analysis for the recommended reconstitution buffer formulation.
We do not conduct Michaelis-Menten studies or determine Km values for our enzymes. Our activity specification is specific activity as measured under the described conditions on the product datasheet.
Some R&D Systems proteins are expressed as chimeras fused to the Fc fragment of an IgG antibody. This can offer advantages for certain proteins. For instance, the Fc portion might stabilize the molecule. In addition, biologically active dimeric proteins can be created by using the natural tendency of the Fc portion to dimerize. Receptor-Fc fusions can also result in a recombinant receptor with higher affinity for its ligand compared to the soluble receptor alone. R&D Systems offers the same recombinant Fc portion separately for use as a control (Recombinant Human IgG Fc; Catalog # 110-HG or Recombinant Mouse IgG2A Fc; Catalog # 4460-MG).
Proteins should always be reconstituted and stored with the buffer recommended on the datasheet. Some proteins are extremely hydrophobic at neutral pH. If the suggested buffer is not used to reconstitute these proteins, they do not go fully into solution and much of the material may cling to the sides of the vial. When the protein is used for an assay, it can be diluted to working concentration with media or another suitable buffer which will neutralize the small amount of acid and make it safe to use with live cells.
The additional BSA in the reconstitution buffer will aid in the recovery and stability of the protein. The volume of PBS in which the product is lyophilized is generally very small. Therefore, PBS reconstitution does not significantly increase the salt concentration when reconstituted according to the datasheet. The presence of additional salt in the stock does not interfere in an assay when diluted to the working concentration. Please contact Technical Service if the volume of PBS prior to lyophilization is a concern. Because products are Quality Control tested in the manner stated on the datasheet, R&D Systems cannot guarantee the performance of products not reconstituted as described.
We generally have not seen adverse effects in our bioassays or other approved applications. However, customers are advised to run a control in their assay to determine if the concentration of trehalose in the protein or antibody formulation has any adverse effects.
Trehalose is a non-reducing sugar and does not react with amino acids or proteins as part of the Maillard reaction. It is added to stabilize antibodies and other proteins against damage caused by freezing. It can also make proteins more resistant to moisture when lyophilized, resulting in a product that is less likely to precipitate when reconstituted.
Often the sequence, the expression system, and the basic manufacturing SOP for traditional and GMP proteins are the same. This makes the transition from using research-use proteins to GMP as seamless as possible. In addition, compared to traditional proteins, GMP proteins come with extensive documentation for traceability as well as additional quality control testing and quality assurance review.An overview of R&D Systems' GMP-grade Proteins can be found on the web site: https://www.rndsystems.com/products/good-manufacturing-practices-gmp-grade-proteins