Spectrophotometric determination of platelet counts in platelet-rich plasma

被引:14
|
作者
Kitamura, Yutaka [1 ]
Suzuki, Masashi [1 ]
Tsukioka, Tsuneyuki [1 ]
Isobe, Kazushige [1 ]
Tsujino, Tetsuhiro [1 ]
Watanabe, Taisuke [1 ]
Watanabe, Takao [1 ]
Okudera, Hajime [1 ]
Nakata, Koh [2 ]
Tanaka, Takaaki [3 ]
Kawase, Tomoyuki [4 ]
机构
[1] Tokyo Plast Dent Soc, Kita Ku, Tokyo, Japan
[2] Niigata Univ Med & Dent Hosp, Biosci Med Res Ctr, Niigata, Japan
[3] Niigata Univ, Dept Mat Sci & Technol, Niigata, Japan
[4] Niigata Univ, Inst Med & Dent, Div Oral Bioengn, Niigata, Japan
关键词
Platelet; Count; Spectrophotometry; Leukocytes; Red blood cells; Quality assurance; GROWTH-FACTOR; LYMPHOCYTE RATIO; METAANALYSIS; NEUTROPHIL;
D O I
10.1186/s40729-018-0140-8
中图分类号
R78 [口腔科学];
学科分类号
1003 ;
摘要
Background: Platelet-rich plasma (PRP) is widely used in regenerative dentistry and other medical fields. However, its effectiveness has often been questioned. For better evaluation, the quality of individual PRP preparations should be assured prior to use. We proposed a spectrophotometric method for determination of platelet counts and validated its applicability using two types of PRP preparations. Methods: Blood samples were obtained from healthy male volunteers and pure PRP (P-PRP) and leukocytes-rich PRP (L-PRP) were prepared using the double-spin method. In serial dilutions, platelet counts in P-PRP and L-PRP were determined using an automated hematology analyzer and a compact spectrophotometer. For validation, PPRP and L-PRP independently prepared by three well-trained operators were used for comparison of the calculated and measured platelet counts. Results: In the two types of PRP samples evaluated, platelet counts were almost equal and greater amount of both white blood cells (WBCs) and red blood cells (RBCs) were included in L-PRP preparations. The calibration curve obtained from serially diluted P-PRP showed a strong correlation (R-2 = 0.995), whereas that of L-PRP was relatively weaker (R-2 = 0.975). In validation testing, the scatter plot of the calculated platelet counts versus the measured values showed a strong correlation in P-PRP (R-2 = 0.671), whereas that of L-PRP showed a much weaker correlation (R-2 = 0.0605). Conclusions: This method can precisely determine platelet counts in PRP preparations when the inclusion of WBCs or RBCs is minimized. Therefore, we recommend that clinicians use this method for quality assurance of individual PRP preparations.
引用
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页数:8
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