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Vacuum-Blood-Collection静脉采血英文课件.ppt

1、Vacuum Blood Collection IntroductionThe vacuum blood collection system consists of a double-pointed needle,a plastic holder or adapter,and a series of vacuum tubes with rubber stoppers of various colors.The evacuated tube collection system will produce the best blood samples for analysis.The blood g

2、oes directly from the patient vein into the appropriate test tube.Multi-Sample NeedleThe bevel is the slanted opening at the end of the needle.Needle length(shaft)ranges from 1 to 1 inches.Threaded hub screws into needle holderThe rubber sheath makes it possible to draw several tubes of blood by pre

3、venting leakage of blood as tubes are changed.BevelBevel is slanted opening at end of needle.Needle must be oriented so that bevel faces up prior to insertion.Needle GaugeThe gauge of a needle is a number that indicates the diameter of its lumen.The lumen,also called the bore,is the circular hollow

4、space inside the needle.The higher the gauge,the smaller the lumen.The most frequently used gauges for phlebotomy are 20,21 and 22HolderThe holder for vacuum blood collection is a plastic sleeve into which the phlebotomist screws the double pointed needle.The most current guidelines require that all

5、 holders are for single use only.Vacuum Collection TubesVacuum collection tubes are glass or plastic tubes sealed with a partial vacuum inside by rubber stoppers.The air pressure inside the tube is negative,less than the normal environment.After inserting the longer needle into the vein,the phleboto

6、mist pushes the tube into the holder so that the shorter needle pierces the stopper.The difference in pressure between the inside of the tube and the vein causes blood to fill the tube.The tubes are available in various sizes for adult and pediatric phlebotomiesAdditivesDifferent blood tests require

7、s different types of blood specimens.Most tubes have additives called anticoagulants which prevent clotting/coagulation of the blood.Plastic tubes may have an additive to enhance clotting of the bloodAnticoagulantsAnticoagulants are already in the tubes in the precise amount needed to mix with the a

8、mount of blood that will fill the tube.The color of the stopper on each tube indicates what,if any,anticoagulant the tube contains.It is important to completely fill each tube so that the proportion of blood to chemical additive is correct,otherwise,the test results may not be accurate or the specim

9、en will be rejected and will need to be recollected.It is also important to thoroughly mix the blood with the additive by gentle inversionRedNo additive in glass tubeClot activator in plastic tubeNo anticoagulant presentTests using serum which include:most blood chemistries,AIDS antibody,viral studi

10、es,serology tests,Blood Bank testing.Red and black mottled(SST)Hemogard=GoldSST=Serum Separator Tube silicone/gel(serum separating material)All tests using serum except Blood BankRed and black mottled(SST)Using BD SST TubesPurpose of gel is to separate serum from cells permanently(Light)BlueAdditive

11、-Sodium CitrateTests drawn:Coagulation studies:PT,PTT and fibrinogenMUST BE FILLED COMPLETELY!NO EXCEPTIONSLavender Top TubeAdditive=EDTA(ethylenediaminetetraacetic)Hematology studies:CBC,WBC count,Hemoglobin,Hematocrit,Platelet count,Reticulocyte count,differential.GreenOne of the following:sodium

12、heparin,lithium heparin or ammonium heparin.STAT blood chemistries utilizing plasma.Green PSTAdditive is heparinPST=Plasma Separator TubeHas gel which,after centrifugation,permanently separates plasma from red blood cellsGrayAdditive(read label):Potassium oxalate and sodium fluoride,or lithium iodac

13、etate and heparinGlucose,Blood Alcohol(ethanol)levels,lactic acidBlackBuffered Sodium CitrateWestergren sedimentation rate determinationMUST BE FILLED COMPLETELY!NO EXCEPTIONSRoyal BlueColor of tube label indicates additive,if any:purple-EDTAgreen-heparinred none Trace metal analysis,nutrients and t

14、oxicology studies.Antimony Arsenic,Cadmium,Calcium,Chromium,Copper,Iron,Lead,Magnesium,Manganese,and Zinc are examples.Brown/TanAdditive=Sodium Heparin or K2 EDTASpecifically for lead analysis although royal blue can be used.YellowSodium polyanethol sulfonate(SPS)SPS for blood culture specimen colle

15、ctions in microbiology.Tube inversions prevent clotting.Acid citrate dextrose additives(ACD)ACD for use in blood bank studies,HLA phenotyping,DNA and paternity testing.Blood CulturesNot for laboratory analysis,special collection to detect bacteria growing in blood.Site preparation VERY important.Wil

16、l be covered later.Order of the Draw1.Sterile/Blood cultures2.Blue coagulation tube3.Red4.Other additivesGreenLavenderGrayPatient IdentificationIt is vitally important that the phlebotomist correctly identifies the patient.Do not offer the patient a name to respond to.All hospitalized patients have

17、an identification arm band with their name,hospital identification number and other pertinent information.Always compare the laboratory test request slip name and ID number with the name and ID number on the patients hospital arm band.If there is any discrepancy,do not draw the patients blood.For an

18、 out-patient,verify the patients identity by having the patient give you additional identifying information such as a social security number,date of birth or address.Preparationwash or disinfect his or her hands Identify patientIntroduce yourself,state your missionHave you ever had your blood drawn

19、before?If no,explain the procedureChoose the appropriate tubes for the tests requested Tourniquet ApplicationApply approximately 3-5 inches above antecubital fossa.If the skin appears blanched above and below the tourniquet it is too tight.If your finger can be inserted between the tourniquet and th

20、e patients skin it is too loose.PalpateAfter tourniquet application have patient clench fist.Feel for a vein that rebounds(bounces)when pushed or tapped on.PALPATE any potential vein to help determine size,direction and depth.A slight rotation of the arm may help to better expose a vein that may oth

21、erwise be hidden.Vein SelectionChoose the veins that are large and accessible.Large veins that are not well anchored in tissue frequently roll,so if you choose one,be sure to secure it with the thumb of your nondominant hand when you penetrate it with the needle.Avoid bruised and scarred areas.Cant

22、Feel the Vein?Tricks to Help Distend Veins:Have the patient pump the hand 3 times.Dont overdue it because over-pumping can create hemoconcentration Have the patient dangle arm below the heart level for 1-3 minutes.Warm the area with a hot pack or warm,moist cloth heated to approximately 42C.If all e

23、lse fails,consult another technician for their opinion and/or intervention.Selection of VeinVeins for VenipunctureVeins used for drawing blood1.Median cubital vein-first choice,well supported,least apt to roll2.Cephalic vein-second choice3.Basilic vein-third choice,often the most prominent vein,but

24、it tends to roll easily and makes venipuncture difficultMedian Cubital first choiceThis vein is located in the antecubital fossa.(the area of the arm in front of the elbow)Well anchored vein,usually large and prominent.Very few problems.Offering the best chance for a close to painless puncture,as th

25、ere are few nerve endings close to this vein.Cephalic Vein-Second ChoiceCephalic vein which is located on the upper or shoulder side of the arm.This vein is usually well anchored.The cephalic vein may lie close to the surface.A low angle of needle insertion must be used to avoid possible spurting or

26、 blood forming a drop at the puncture site.(15)Basilic Vein-Third ChoiceLocated on the under side of the arm.In many patients this vein may not be well anchored and will roll,making it difficult to access with the needle.Syringe draw should be considered as it gives the phlebotomist more control ove

27、r a rolling vein.Pooling of blood and hematoma formation possible.The basilic vein is close to the brachial artery so there is more risk of hitting an artery.Exercise caution when drawing from this area.Additionally,this area is often more sensitive,thus a stick is slightly more painful for the pati

28、ent Cleansing the SiteAfter selecting a vein,clean the puncture site with a cotton ball saturated with 70%isopropyl alcohol or prepackage alcohol swabs.Rub the alcohol swab in a circular motion moving outward from the site Use enough pressure to remove all perspiration and dirt from the puncture sit

29、e.Discreetly look at the swab when finished,if it appears excessively dirty repeat the cleansing process with a fresh alcohol swab.After cleansing do not touch the site,if the vein must be repalpated the area must be cleansed again.Some experts allow cleansing of the index finger before repalpating

30、but this technique is debatable.Assemble EquipmentTwist needle into holder.Select appropriate tubes and insert first tube into holder.DO NOT remove cap until right before you are ready to stick.Re-Apply Tourniquet and Prepare to StickPerforming the StickHold the prepared holder with the bevel up.Use

31、 the thumb of the nondominant hand below the puncture site to anchor the vein and pull the skin taut.The needle entering the site should not touch the thumb of the phlebotomist.Position the needle in the same direction as the vein,enter the skin and penetrate the vein at a 15 degree angle in one swi

32、ft,smooth motion to decrease the patients discomfort.If you enter to slowly blood will leak out at the puncture site creating a biological hazard as well as obstructing your view of the puncture site.The bevel of the needle should enter and remain in the center of the vein.Performing the DrawEnding

33、Draw-Release TourniquetTourniquet cannot be in place more than 1 minute.Release the tourniquet as the last tube is filling.Use one handed method of release.Ending DrawRelease last tube from needle.Hold gauze sponge or biowipe above needle.Swiftly withdraw needle.As soon as needle is withdrawn apply

34、pressure to puncture site.If possible,have patient continue to apply pressure.Ending the Draw TTNActivating Safety DeviceAs soon as you remove needle and apply pressure activate the safety device.DO NOT USE YOUR OTHER HAND TO SNAP DEVICE INTO PLACEEVER!Needle DisposalAs soon as needle safety device

35、is activated dispose of entire assembly in a biohazard sharps container.Labeling TubesLabel all tubes appropriately at the patients side.Do not take unlabeled tubes from the patients presence.Minimum information:Patients full name,last name firstID numberDate,time and your initialsChecking SiteGentl

36、y remove gauze or biowipe.Inspect area for continued bleeding or swelling.If all ok place bandaid over site.Tell patient to remove in 10-15 minutes.If patient still bleeding DO NOT leave,continue to apply pressure.Leaving Discard all used materials hint-place all wrappers,alcohol swab,needle cap in

37、palm of gloved hand,remove glove.Thank patient.Wash hands.LeaveBD EclipseThe BD Vacutainer Eclipse Blood Collection Needle is a safety-engineered multi-sample blood collection needle.It features a patented safety shield that allows for one-handed activation to cover the needle immediately upon withd

38、rawal from the vein and confirms proper activation with an audible click We will use this device next week.Problems with Needle InsertionProblems with Needle InsertionSources of Error1.Failure to insert the needle completely into the vein.The phlebotomist should feel resistance initially following i

39、nsertion of the needle.The resistance is almost immediately followed by a sensation of free or easier movement as the needle enters the vein.Puncturing the stopper before entering the vein.If the phlebotomist partially pushes the evacuated tube onto the needle before inserting the needle into the ve

40、in,he/she risks puncturing the stopper and releasing the vacuum.2.Not anchoring the vein before inserting the needle.The vein must be held in place for successful needle penetration.3.Bouncing the needle on the skin before guiding it into the vein.During venipuncture,the patient should only be stuck

41、 once with the needle.4.Not keeping the holder stationary,causing the needle to dislodge from the vein.Rejection of Samples1.Hemolysis-this is usually caused by a procedural error such as using too small of a needle,or pulling back to hard on the plunger of a syringe used for collecting the sample.T

42、he red cells rupture resulting in hemoglobin being released into the serum/plasma,making the sample unsuitable for many laboratory tests.The serum/plasma will appear red instead of straw colored.Rejection of Samples1.Clotted-failure to mix or inadequate mixing of samples collected into an additive t

43、ube.The red cells clump together making the sample unsuitable for testing.2.Insufficient sample(QNS)-certain additive tubes must be filled completely.Incorrect blood to additive ratio will adversely affect the laboratory test results.When many tests are ordered on the same tube be sure to know the a

44、mount of sample needed for each test.3.Wrong tube collected for test ordered.Always refer to procedure manual when uncertain.4.Improper storage-certain tests must be collected and placed in ice,protected from light,or be kept warm after collection.5.Improperly labeled First Aid Following Needlestick

45、Regardless of the disease the patient has,be careful not to stick yourself with a used needle.If an accidental stick does happen,immediately nGo to the sink,turn on the water,and bleed the site well by alternating squeezing and releasing the area around the site.nDo this for approximately 3 to 5 minutes.nAfterwards scrub the site with an alcohol swab.nFollow with a thorough hand washing.Report it to your instructor immediately.

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