Red Blood Cells
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»Red Blood Cells is the portion of blood that contains hemoglobin and is derived from human whole blood,from which plasma and platelets are removed by centrifugation,sedimentation,or by apheresis.In the case of apheresis,the plasma is automatically removed and returned directly to the donor.Red Blood Cells derived from whole blood may be prepared at any time during the dating period of the whole blood from which it is derived.
Red Blood Cells may be further processed by addition of red cell preservatives,irradiation to inactivate lymphocytes,filtration for removal of leukocytes,washing to remove proteins,freezing and thawing,or rejuvenation using validated and approved procedures.The source blood for Red Blood Cells must be tested for syphilis,hepatitis Bvirus,hepatitis Cvirus,human T-cell lymphotropic virus (HTLV)type Iand type II,human immunodeficiency virus (HIV)type 1and type 2,and unexpected antibodies to red cell antigens using FDA-approved and licensed commercially available test kits,the results of which must be below the limits of detection specified in the respective test kits by the manufacturers.In addition,the source blood must also be tested for hepatitis Cand HIVusing FDA-approved nucleic acid assays,the results of which must be below the approved limits of detection for the method.Aunit (dose)of Red Blood Cells contains a minimum of 50g of hemoglobin in a total volume of approximately 180to 325mL.Aunit (dose)of Red Blood Cells,Leukocytes Reduced contains a minimum of 42.5g of hemoglobin in a total volume of approximately 150to 275mL,and has a residual leukocyte count of less than 5×106.Aunit (dose)of Red Blood Cells,Deglycerolized contains a minimum of 40g of hemoglobin in a total volume of approximately 180to 325mL.Aunit (dose)of Red Blood Cells,Leukocytes Reduced and Deglycerolized contains a minimum of 34g of hemoglobin in a total volume of approximately 180to 325mLand has a residual leukocyte count of less than 5×106.Aunit (dose)of Red Blood Cells,Pheresis contains a mean hemoglobin content of 60g of hemoglobin.Aunit (dose)of Red Blood Cells,Pheresis,Leucocytes Reduced contains a mean hemoglobin content of 51g (or 153-mLpacked red cell volume,and has a residual leukocyte count of less than 5×106.USP28
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Packaging and storage
Collect into an approved container (see Transfusion and Infusion Assemblies á161ñ)containing a sterile,pyrogen-free approved anticoagulant (see Anticoagulant Citrate Dextrose Solution,Anticoagulant Citrate Phosphate Dextrose,or Anticoagulant Citrate Phosphate Dextrose Adenine Solution).An approved additive solution may be added after removal of the plasma.Store Red Blood Cells in the original container,or transfer to an equivalent container using a technique that does not compromise sterility.Liquid Red Blood Cells is stored at a temperature between 1and 6(see General Notices and Requirements).Frozen Red Blood Cells is stored at 65or colder.USP28
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Expiration date
Red Blood Cells in Anticoagulant Citrate Dextrose Solution,Anticoagulant Citrate Phosphate Dextrose Solution,or in Anticoagulant Citrate Phosphate Dextrose-Dextrose Solutionmay be stored for up to 21days at 1to 6after the blood has been drawn.Red Blood Cells in Anticoagulant Citrate Phosphate Dextrose Adenine Solutionmay be stored for up to 35days at 1to 6.Red Blood Cells may be stored in an approved additive solution (AS),*for up to 42days at 1to 6.If the hermetic seal of the container is broken during collection,preparation,or further processing,the expiration date is not later than 24hours after the seal is broken (when blood is stored at 1to 6).The expiration date for frozen Red Blood Cells prepared with low glycerol content (20%glycerol)is not later than 10years from the date of collection when stored at 120or colder,except when Red Blood Cells is prepared for freezing with high glycerol content (40%glycerol),in which case it may be stored at 65or colder for no later than 10years from date of collection.If the frozen Red Blood Cells is processed for freezing or for thawing,in an open system,the expiration date for the thawed Red Blood Cells is 24hours after removal from 65storage,provided it is then stored at the temperature of unfrozen Red Blood Cells.USP28
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Labeling
Label the container to indicate the volume of the whole human blood collected from the donor,the collection date,the donation number or other coding means to uniquely identify the unit and to provide traceability to the donor,and the expiration date.Label it to indicate the type of anticoagulant used to collect whole human blood and any additive solutions added subsequent to collection.Label it also to identify donor status (i.e.,volunteer or paid).Label it also with the following statements:See Circular of Information for indications,contraindications,cautions,and methods of infusion.;Properly identify recipient.;and Caution:Rx only.In addition,label it to indicate the product name as indicated in Table 1.[NOTEThe name is determined by the method of preparation of the Red Blood Cells (derived from whole human blood or from apheresis)and by performing the necessary testing to ensure that the product meets the minimum requirements for the named products,as indicated in Table 1.]
Table 1.Red Blood Cells Preparations
Label it to indicate,the ABO Group/Rh Type,as indicated in Table 2.[NOTEEvery Red Blood Cell product must have a determination made as to its ABO Group and Rh Type and specificity of unexpected red cell antibodies,if any.]
If an ABOblood group color scheme is used,use the following labeling color:Group A(yellow),Group B(pink),Group O(blue),and Group AB(white).
Label the Red Blood Cells with names of the adventitious agents tested and the results of the tests.If it has been issued prior to determination of the test results,label it also with a warning Donor Untestedand to specify Uncrossmatched Blood,when appropriate.
Table 2.Blood Group and Rh Type
Add the following:
Identification
A:ABOblood group
Anti-Areagent
Use approved commercially available monoclonal or polyclonal anti-Ablood grouping reagent,two different lots from the same or different manufacturers.Use in accordance with manufacturer's instructions.
Anti-Breagent
Use approved commercially available monoclonal or polyclonal anti-Bblood grouping reagent,two different lots from the same or different manufacturers.Use in accordance with manufacturer's instructions.
Anti-ABreagent
Use approved commercially available anti-ABblood grouping reagent.Use in accordance with manufacturer's instructions.
Control preparations
On the day of use,dilute Blood Group A1(Control preparation A1)and Blood Group B(Control preparation B)red blood cells,obtained from an approved commercial source or prepared by the testing laboratory,with 0.9%saline to suspensions of approximately the same concentration between 2%to 5%(v/v).[NOTEIf the Blood Group A1and Blood Group Bred blood cells are prepared in the testing laboratory from whole blood of a known blood group,it must be prepared on the day of use following the procedure for the Test preparationunder Whole Blood.]
Test preparation
On the day of use,dilute Red Blood Cells with 0.9%saline to a suspension of about the same concentration as the Control preparations.
Procedure
On a suitable U-bottomed microtiter plate,place 1drop of 0.9%saline in each of three different wells in a row(Blank Row).Place 1drop from one of the lots of Anti-Areagent in each of three different wells in a second row.Place 1drop from the second lot of Anti-Areagent in each of three different wells in a third row.Repeat the same with two different lots of Anti-Breagent and one lot of Anti-ABreagentin separate rows.To each row,add 1drop of Control preparation A1,Control preparation B,and the Test preparationin the first,second,and the third well,respectively,of each row.Mix the contents of the wells by gently tapping the sides of the plate.Centrifuge the plate at the appropriate conditions established for the centrifuge.Resuspend the cell buttons by manually tapping the plate,or with the aid of a suitable mechanical shaker.Read the optical densities at different wells using a suitable automated photometric microtiter plate reader.Compare the optical density of each well in the Blank Row with the optical density of the wells to which the corresponding Control preparation A1,Control preparation B,or Test preparationwere added.[NOTEAhigh optical density comparable to those obtained for the wells in the Blank Rowindicates negative results (no hemagglutination),which can be corroborated by visual observation of smooth suspensions.Alow optical density indicates positive results (hemagglutination),which can be corroborated by visual observation of formation of clumps.]The blood group of Red Blood Cells is A,B,AB,or O,accordingly,as the Test preparationis hemagglutinated by Anti-Areagent,Anti-Breagent,both reagents,or neither,respectively.The blood group of the Test preparationconforms to the blood group indicated on the label.The test is not valid if Control preparationsfor Blood Group Aand Blood Group Bred blood cells are not agglutinated by Anti-Areagentand Anti-Breagent,respectively,or if both Control preparationsare not agglutinated by Anti-ABreagent.The test is also not valid if the Test preparationis not agglutinated by Anti-ABreagentbut is agglutinated by either Anti-Areagentor Anti-Breagent,or is agglutinated by Anti-ABreagentbut not by either Anti-Areagentor Anti-Breagent.
B:Rh type
USP28
TEST1
Anti-D(Rho)reagent
Use anti-D(Rho)blood grouping reagent approved for use in microtiter plate tests.Dilute,if necessary,following the manufacturer's instructions.
Test preparation
On the day of use,dilute Red Blood Cells with 0.9%saline to obtain a 2%to 5%(v/v)suspension.
Procedure
On a suitable U-bottom microtiter plate,place 1drop each of 0.9%saline and Anti-D(Rho)reagent in two separate wells.Label them as the Bwell (Blank)and the Twell,respectively.Add 1drop of Test preparationto each well,and mix by gently tapping the side of the plate.Centrifuge the plate at appropriate conditions established for the centrifuge.Resuspend the cell buttons by manually tapping the plate,or with the aid of a suitable mechanical shaker.Read the optical densities of the wells using a suitable automated photometric microtiter plate reader,and determine if the Red Blood Cells in the Twell is agglutinated as described under Identificationtest A.If the Twell indicates negative results (no hemagglutination),incubate the plate at 37for 15minutes,centrifuge,resuspend the cells,and read the optical densities of the wells as above.Agglutination of cells after immediate-spin or after 37incubation indicates Rh positive typing of Red Blood Cells.The test is valid if cells in the Bwell are not agglutinated.If the cells are not agglutinated in the Twell,proceed as directed in Test 2.
TEST2
Anti-Dreagent
Use anti-Dblood grouping reagent approved for use for a weak Dblood group test.
Antihuman globulin reagent
Use polyspecific or anti-IgGantihuman globulin reagent.Dilute,if necessary,following the manufacturer's instructions.
Control preparation
Use IgG-coated red cells approved for use as a control for Rh typing.Dilute with 0.9%saline to obtain a 2%solution.
Test preparation
Prepare as directed for Test 1.
Procedure
Place 1drop of 0.9%saline into a suitable test tube and 1drop of Anti-Dreagentin another,and mark them as the Blank and Anti-D,respectively.To each tube add 1drop of the Test preparation,mix,and incubate at 37for 15to 30minutes.Centrifuge the tubes at about 1000gfor 15to 30seconds.Gently resuspend the cell buttons,and examine them for hemagglutination (formation of clump)by visual examination.The Rh typing of Red Blood Cells is positive or negative according to whether the cells in Anti-Dtube are agglutinated or not.If the cells are not agglutinated,add 1mLof 0.9%saline to the Anti-Dtube,and resuspend the cells.Centrifuge the tube at about 1000g for 1minute,and remove the saline completely.Repeat the step two to three times more to wash the Red Blood Cells.Add 1drop of 0.9%saline and 1to 2drops of Antihuman globulin reagentto the Anti-Dtube.Mix gently,and centrifuge the tube at about 1000gfor 15to 30seconds.Gently resuspend the cell button,add 1drop of Control preparation,mix gently,centrifuge as above,and examine for agglutination.The Rh Type of the Test preparationconforms to the Rh Type indicated on the label.The test is not valid if the cells in the Anti-Dtube are not agglutinated after addition of the Control preparation.Also,for the test to be valid,the cells in the Blank tube must not be agglutinated.
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Visual inspection
Inspect visually during storage and immediately prior to use.If the color or physical appearance is abnormal or there is any indication or suspicion of microbial contamination,the unit is unsuitable for transfusion.USP28
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Hemoglobin content
Drabkin's solution
Dissolve Drabkin's reagent in a suitable volume of water,and add a suitable volume of a 30%(w/v)polyoxyethylene (23)lauryl ether solution such that the final concentrations of potassium cyanide,potassium ferrocyanide,and polyoxyethylene (23)lauryl ether in the solution are approximately 0.75mM,0.6mM,and 0.015%,respectively.Store the solution in the dark between 18to 26.[CautionDrabkin's reagent and Drabkin's solution contain cyanide and are HIGHLY TOXIC.Do not inhale or swallow or allow contact with skin or with eyes.Wear suitable protective clothing,gloves,and eye and face protection.Do not mix with acids.Contact with acids liberates a very toxic gas.If ingested,perform gastric lavage,and immediately call a physician.
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Blank solution:
water.
Standard solution A
Transfer about 300mg USP Hemoglobin RS,accurately weighed,to a 2-mLvolumetric tube,add 1mLwater,dissolve in and dilute with water to volume,and mix.
Standard solution B
Mix 50µLof Standard solution Awith 25µLof water.
Standard solution C
Mix 50µLof Standard solution Awith 100µLof water.
Test solution
Mix 50µLof Red Blood Cells with 50µLof water.
Procedure
Label suitable tubes as B1,B2,SA1,SA2,SB1,SB2,SC1,SC2,T1,and T2.Add 5.0mLof Drabkin's solution to each tube.Add 20µLof water to each of B1and B2,20µLof Standard solution Ato each of SA1and SA2,20µLof Standard solution Bto each of SB1and SB2,20µLof Standard solution Cto each of SC1and SC2,and 20µLof Test solutionto each of T1and T2,rinsing the pipet tip three to four times with Drabkin's solution,and mix.Allow to stand for at least 15minutes at room temperature.[NOTERed Blood cells with appreciable carboxyhemoglobin content,such as those obtained from smokers,may require longer reaction time.If the donor characteristics are not known,the incubation time should be optimized prior to testing.]Read the absorbances of the solutions against the solution in tube B1at 540nm.The absorbance of the solution in tube B2is recorded at the end.The test is not valid if the absorbance of the solution in tube B2is not within ±0.005.
Calculations
Calculate the concentrations,in mg per mL,of hemoglobin in Standard solutions A,B,and C.Plot a calibration curve of absorbance values against the hemoglobin concentration by drawing a best-fit straight line using the least-square linear regression analysis.From the absorbance value of the Test solution,obtain the concentration,in mg per mL,of hemoglobin in the Test solution.Multiply the value by 2to obtain the concentration,in mg per mL,of hemoglobin in Red Blood Cells.Calculate the total hemoglobin content in the Red Blood Cells unit,in g,by the formula:
Conc.of hemoglobin (in mg/mL)×the volume of the Red Blood Cells unit (in mL)/103.
USP28
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Leukocyte count
Pipet 40µLof a suitable red cell-lysing agent into a clean test tube,add 100µLof Red Blood Cells diluted with 0.9%saline,if necessary,such that the hematocrit of Red Blood Cells is not greater than 60%.Mix by pipetting up and down several times.Add 360µLof 0.01%(w/v)crystal violet in 15%(v/v)acetic acid into the mixture,and mix thoroughly.Fit a hemocytometer with a 50-µLcounting volume and a bright background,with a cover slip,and load the counting chamber with the mixture until the counting area is completely covered,but not overfull.Cover the counting chamber with a suitable moist lid to prevent evaporation,and allow to settle undisturbed for 10to 15minutes.Remove the lid,place the chamber on the stage of a light microscope fitted with 10×ocular lens and 20×objective.Count the leukocytes in the entire 50-µLcounting volume.Calculate the leukocyte count in Red Blood Cells,expressed in leukocytes per µL,by dividing the observed leukocyte count by 10.Calculate the total number of leukocytes in the Red Blood Cells unit by using the following formula:
Total leukocytes =leukocytes/µL×103×the volume of the Red Blood Cells unit in mL.
USP28
Add the following:
Adequacy of deglycerolization(for Red Blood Cells,Deglycerolized)
Interrupt the last wash cycle of the deglycerolization process at a point where the wash fluid is visible in the clear tubing segment leading to the waste receptacle.Hold the tubing against a well-lighted,white background.Note the coloration of the fluid in the tubing,and compare it to a suitable hemolysis color comparator standard.The color of the fluid should be no stronger than the block indicating 3%hemolysis.[NOTEIf the level of hemolysis is more than 3%,continue the wash process,and repeat the test until the color is within acceptable limits.]USP28
*
AScontains sodium chloride,dextrose,adenine,and other substances that support red cell survival and function.Examples of such solutions are AS-1,AS-3,and AS-5.
Auxiliary Information
Staff Liaison:Radhakrishna S Tirumalai,Scientist
Expert Committee:(BBP)Blood and Blood Products
USP28NF23Page 275
Pharmacopeial Forum:Volume No.30(1)Page 69
Phone Number:1-301-816-8339
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