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Platelet-Derived Microparticels Stimulate Proliferation of Colony-Forming Unit Granulocyte-Macrophage of Umbilical Cord Blood Hematopoietic Stem Cells.

Chen, Bao-An ; Fei, Fei ; Huang, Cheng-Yin ; [et al.]

American Society of Hematology ; 2005

In: Blood Vol. 106, No. 11 ( 2005-11-16), p. 4191-4191

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In: Blood, American Society of Hematology, Vol. 106, No. 11 ( 2005-11-16), p. 4191-4191

Abstract: Umbilical Cord blood has become an important source of hematopoietic stem-progenitor cells for transplantation, however hematopoietic recovery after transplantation with umbilical cord blood is slower than with bone marrow or mobilized peripheral blood. Adhesion molecules on hematopoietic cells are involved in hematopoietic cells’ homing, which is considered the most important step of hematological recovery. Some articles indicated that expressions of adhesion molecules on CD34+ cells could predict the time to hematopoietic recovery after transplantation with bone marrow and peripheral blood of many adhesion molecules (such as CD62, CXCR4) are significantly lower on umbilical cord blood than on bone marrow. It is a possible reason for the difficulty in hematopoietic recovery after umbilical cord blood transplant. Platelet -derived microparticles (PMPs) are submicroscopic ( & lt;1 μm) membrane vesicles released from platelet if they are stimulated with agonists such as thrombin, collagen, or calcium ionophore A23187 or if exposed to high-stress shear forces. PMPs express several platelet-endothelium attachment receptors on their surface, for example, glycoprotein IIb/IIIa (CD41), Ib and IaIIa, and P-selectin (CD62P) and several other platelet relevant receptors such as CXCR4 and PAR-1. Some articles indicate that PMPs can affect the function of hematopoietic stem cells by increasing the adhesion of hematopoietic cells to fibrinogen, which suggests that PMP-transferred CD41 antigen plays an important role in this process. PMPs can also increase the survival of human hematopoietic cells including human CD34+ clonogenic progenitors. In our research, we observe the function of PMP to affect the cloning efficiency of colony-forming unit granulocyte-macrophage (CFU-GM). We adopt different concentrations of Thrombin (2U/ml, 1.5U/ml, 1.0U/ml and 0.5U/ml) to activate the platelet and acquire PMPs. Then PMPs were evaluated by using flow cytometry. Based on the result that stimulation of platelets by Thrombin (1U/ml) can acquire the best efficiency of PMPs, we used this concentration in all subsequent experiments. Umbilical cord mononuclear cells (MNCs) were obtained from healthy donors and isolate the MNCs by Ficoll-Hypaque density gradient centrifugation. Briefly, MNCs incubated with or without PMPs cultured in 2.7% methylcellulose. CFU-GM growth was stimulated with 30% umbilical cord serum, rhIL-3 and rh GM-CSF. Cultures were incubated at 37°C in a fully humidified atmosphere supplemented with 5% CO2. Colonies were counted under an inverted microscope after 7 or 10 days. The research was divided into four groups: 1. control group; 2. PMPs(10μg/ml); 3. PMPs(50μg/ml); 4. PMPs(100μg/ml). The colony formation was enhanced with PMPs and is dependently stimulated with PMPs. The number of colonies in the group of PMPs(100μg/ml) is more than that of other groups. The number of colonies in control group, PMPs(10μg/ml), PMPs(50μg/ml) and PMPs(100μg/ml) are 57.4±3.2, 65.6±5.6, 77.1±1.7 and 87.8±5.0 per 1×105 respectively. These increases in different groups were statistically significant when compared with control group(p & lt;0.05). To sum up, PMPs can affect the cloning efficiency of CFU-GM of umbilical cord hematopoietic stem cells and the efficiencies are depended on the concentration of PMPs.

Type of Medium: Online Resource

ISSN: 0006-4971 , 1528-0020

URL: Article

DOI: 10.1182/blood.V106.11.4191.4191

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XA 33000

RVK:

XA 10000

Language: English

Publisher: American Society of Hematology

Publication Date: 2005

detail.hit.zdb_id: 1468538-3

detail.hit.zdb_id: 80069-7

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Platelet-Derived Microparticles Induce Angiogenesis In Vitro and In Vivo.

Chen, Bao-An ; Zhong, Yue-Jiao ; Huang, Cheng-Yin ; [et al.]

American Society of Hematology ; 2007

In: Blood Vol. 110, No. 11 ( 2007-11-16), p. 3901-3901

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In: Blood, American Society of Hematology, Vol. 110, No. 11 ( 2007-11-16), p. 3901-3901

Abstract: Objective: An attempt was made to investigate the effect of platelet-derived microparticles (PMPs) on the angiogenesis. Methods: Thrombin was adopted to activate the platelets to release PMPs. Flow cytometry(FCM)was adopted to evaluate the efficiencies of different concentrations of thrombin to produce PMPs and BCA was adopted to evaluate the content of PMPs. By the carrier of human umbilical vein cell line ECV-304 cultivated in vitro, investigate the effect of PMPs on the proliferation and apoptosis of human umbilical vein endothelial cells using MTT and FCM. PMPs were put into CAM and observe the effects of PMPs on angiogenesis in Chick embryo chorioallantoic membrane (CAM). Results: The efficiencies of PMPs activated by 1.0U/ml thrombin were 50.1%; PMPs induced proliferation of human umbilical vein cell line ECV-304 in a dose dependent manner. At the concentration of 40ug/ml PMPs, the proliferation rate of human umbilical vein cell line ECV-304 was as 1.8±0.3 times as control and there was no difference with the group of vascular endothelial growth factor (VEGF),which the proliferation rate was 1.9±0.5 times vs. control, p & gt; 0.05;PMPs inhibited human umbilical vein cell line ECV-304 apoptosis. Compared with control group (apoptosis rate 9.4%±0.5%), apoptosis rate of PMPs (40μg/ml) is 3.9%±0.4%, which was significantly reduced, p & lt;0.05. The addition of VEGF (10μl/ml) did not successfully prevented apoptosis of human umbilical vein cell line ECV-304 (apoptosis rate 8.0%±0.8%);After 72 h of incubation, showing an implant of PMPs by allantoic vessels developing radially towards it (implant) in a ’spoked-wheel’ pattern, at the concentration of 80μg/ml PMPs, number of vessel ramification is 112.5±11.31 and vessel area/CAM area is (6.19±1.29)%, compared with the VEGF(p & gt;0.05). But there are not localized allantoic vessels developing in the NS control group(P & lt;0.05). Conclusion: 1.0U/ml thrombin activated platelet could get the best efficiency of PMPs, which could stimulate proliferation of human umbilical vein cell line ECV-304 and inhibit its apoptosis and PMPs have certain promotive effect on the formation of capillary in chick chorioallantoic membranes.

Type of Medium: Online Resource

ISSN: 0006-4971 , 1528-0020

URL: Article

DOI: 10.1182/blood.V110.11.3901.3901

RVK:

XA 33000

RVK:

XA 10000

Language: English

Publisher: American Society of Hematology

Publication Date: 2007

detail.hit.zdb_id: 1468538-3

detail.hit.zdb_id: 80069-7

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Building and Clinical Use of Activated Plasma Clotting Time Test and the Value of APCT on Predicting the Bleeding Due to Leukemia Chemotherapy-Induced Thrombocytopenia.

Chen, Bao-An ; Li, Jin-Jin ; Huang, Cheng-Yin ; [et al.]

American Society of Hematology ; 2007

In: Blood Vol. 110, No. 11 ( 2007-11-16), p. 3915-3915

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In: Blood, American Society of Hematology, Vol. 110, No. 11 ( 2007-11-16), p. 3915-3915

Abstract: Objective This study was aimed to determine the optimal concertration of C-PG in activated plasma clotting time (APCT) test and build the APCT test.To investigate the value of activated plasma clotting time test (APCT) on predicting the bleeding due to Leukemia chemotherapy-induced thrombocytopenia. Method We collected healthy blood donors’venous blood, prepared watched platelet suspension and platelet rich plasma in a normal way to which we add different concertrations of C-PG, then test expression of AnnexinV in the surface of activated platelet by FCM. Prepared platelet rich plasma and platelet poor plasma in a normal way to which we add different concertrations of C-PG, then count the plasma clotting time.Forty-one patients with leukemia chemotherapy, twenty-one patients with petechiae or epistaxis or gum bleeding and twenty patients without bleeding symptoms, were involved in the test. Drawed their venous blood and collected in 3.2% buffered sodium citrate(9:1), the platelet counts and APCT, PT, APTT, TT, Fig were assesed. Result Bleeding group’s APCT was obviously prolonged contrast to the non-bleeding group’s. Platelet counts and APCT of the bleeding group and the non-bleeding group were (7.2±2.9) ×109/L, (105.9±8.1)s and (23.0±12.2) ×109/L,(71.4±9.0)s respectively. There was significant difference between the two groups (P & lt;0.01). Using APCT≥90s as the cut-off point to predict the bleeding caused by chemotherapy-induced thrombocytopenia, the sensibility was 100%, and the specificity was 95.7%. Using platelet counts ≤15*109/L, the sensibility and the specificity was 95.2% and 69.0%. PT, APTT, TT, Fig of the bleeding group and the non-bleeding group were 11.7±1.1)S,(31.5±1.3)S,(11.1±1.2)S,(2.37±0.41)g/L and (12.1±0.8)S,(30.8±2.1)S,(10.7±0.9)S,(2.64±0.27)g/L respectively. The results of the two groups were all not significantly different (P & gt;0.05). Conclusion APCT is a good indication of predicting the bleeding due to leukemia chemotherapy -induced thrombocytopenia.

Type of Medium: Online Resource

ISSN: 0006-4971 , 1528-0020

URL: Article

DOI: 10.1182/blood.V110.11.3915.3915

RVK:

XA 33000

RVK:

XA 10000

Language: English

Publisher: American Society of Hematology

Publication Date: 2007

detail.hit.zdb_id: 1468538-3

detail.hit.zdb_id: 80069-7

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Effects of Amifostine and Fengling Polysaccharide on Proliferation and Chemoprotection of Human Granulocyte-Macrophage Progenitor Cells.

Chen, Bao-An ; Huang, Cheng-Yin ; Li, Chui-Ping ; [et al.]

American Society of Hematology ; 2005

In: Blood Vol. 106, No. 11 ( 2005-11-16), p. 4190-4190

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In: Blood, American Society of Hematology, Vol. 106, No. 11 ( 2005-11-16), p. 4190-4190

Abstract: Objective: This paper is to study the proliferation and chemoprotection effects of amifostine (WR-2721) and fengling polysaccharide (FLPS) on the human granulocyte-macrophage progenitor cells. Method: (1) Mononuclear cells (MNC) were deparated by Ficoll (1.077g/ml). The MNC of WR-2721 and FLPS treatment were cultured in methylcellulose senisolid medium, the colony forming unit-granulocyte macrophage(CFU-GM) was measured. The effects of WR-2721 and FLPS on CFU-GM were studied. (2) MNC of WR-2721 treatment or containing FLPS were cultured 14h at 37°C with VP16. The cytoprotective activity against VP16 toxic effects of WR-2721 and FLPS on CFU-GM were observed. (3)To study the effects of WR-2721 on proliferation inhibition and apoptosis of HL-60 human leukemia cell line, the cell apoptosis rate of HL-60 was determined by annexinV/PI double staining method, cell proliferation and chemotherapy sensitivity were analyzed with XTT assay, and the changes of cell cycle were observed through flow cytometry.(4) HL-60 cells of containing FLPS were cultured 14h at 37°C with VP16. The cytoprotective activity against VP16 toxic effects of FLPS on HL-60 cells were observed. Results: (1) The number of CFU-GM was significantly increased in 10 groups by addition of 0.5–25μg/ml FLPS and 12 groups treated with 0.01–5mmol/L WR-2721( 30 min, 37°C), p & lt;0.05. The mean value of CFU-GM in groups of negative control, WR-2721 (1mmol/L), FLPS(5μg/ml) and WR-2721+FLPS were 91.4±50.4,119.8±62.9,143.2±76.4 and 179.2±97.6 per 1×105, respectively, Compared with control, singnificant differences were seen between each group, p & lt;0.05. WR-2721+FLPS group compared with WR-2721 and FLPS group, p & lt;0.01 and p & lt;0.05. (2) The number of CFU-GM was significantly increased in MNC of adding FLPS or WR-2721 treatment. The mean value of CFU-GM in groups of VP-16 control, negative control, WR-2721 + VP16, FLPS + VP-16 and WR-2721 + FLPS + VP16 were 30.9±22.5, 83.2±43.8, 64.6±41.2, 55.3±33.5 and 78.3±48.2 per 1×105, respectively. Compared with VP16 control group, singnificant differences were seen between each group, p & lt; 0.01. (3) After treatment (30min,37°C)with WR-2721, the sensitivity of HL-60 cells to VP-16 was enhanced, and the IC50 descended from 52.5μg/ml to 40.5μg/ml. After 72hours trentment of HL-60 cells with WR-2721, the early apoptotic cells (annexinV-FITC positive/PI negative) were increased from(5.5±1.9)% to (48.5±8.4)%(p & lt;0.001), late apoptotic cells(annexinV-FITC positive/PI positive)were increased from(1.2±0.5)% to (39.0±4.0)% (p & lt;0.001), and HL-60cells were arrested in G2-M phase. (4) HL60 cells were cultured 14h at 37°C with 20μg/ml VP16 and 50μg/ml FLPS, the cell survival rate was 88.0%±2.3%, negetive control was 90.5%±2.9%, no singnificant difference was seen between two group, n =21, p & gt;0.05. Conclusion :(1) WR-2721 and FLPS can increase the prolification of CFU-GM. Combination of WR-2721 and FLPS show stronger effect than the WR-2721 or FLPS alone. (2) WR-2721 and FLPS selectiveiy protect human peripheral blood CFU-GM from the cytotoxicity of VP16 without decreasing its cytotoxic effect on HL60 cells. (3) WR-2721 treatment can enhance HL-60 cells chemotherapy sensitivity to VP-16, inhibit proliferation, induce HL-60 cells apoptosis and accumulation of cells in G2-M phase.

Type of Medium: Online Resource

ISSN: 0006-4971 , 1528-0020

URL: Article

DOI: 10.1182/blood.V106.11.4190.4190

RVK:

XA 33000

RVK:

XA 10000

Language: English

Publisher: American Society of Hematology

Publication Date: 2005

detail.hit.zdb_id: 1468538-3

detail.hit.zdb_id: 80069-7

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Functions of Glycosylation Cooled Rabbit Platelets In Vivo and In Vitro.

Chen, Bao-An ; Huang, Cheng-Yin ; Pei, Xiao-Ping ; [et al.]

American Society of Hematology ; 2006

In: Blood Vol. 108, No. 11 ( 2006-11-16), p. 3902-3902

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In: Blood, American Society of Hematology, Vol. 108, No. 11 ( 2006-11-16), p. 3902-3902

Abstract: This study was aimed to investigate functions of glycosylation cooled rabbit platelets in vivo and in vitro and the method to store cold platelets with UDP-gal. We collected rabbit heart blood, prepared concentrated platelet suspensions in a normal way to which we added UDP-Gal, and then stored them for ten days in 4° refrigerator. Thereafter platelet counts, mean platelet volume, platelet distributing width, platelet aggregation function, the activity to urge coagulation including PF3aT and APCT and apoptosis were determine- d. Meanwhile, survival time in vivo was tested after cold-stored rabbit platelets labeled with Cr51 were transfused into rabbits. Rabbit ear bleeding time and percentage plate recovery(PPR) were determined 1 hour and 24 hour after they were transfused into rabbit thrombocytopenia model. Results show that there was not significant difference in PLT counts, MPV, PDW, PF3aT and APCT between UDP-Gal cold-stored platelet group and fresh platelet group(p 〉 0.05). On the contrary, platelet counts decreased significantly, MPV, PDW jumped and PF3aT and APCT went down in cold control group compared to fresh platelet group(p 〈 0.01). Apoptosis increase in UDP-Gal cold-stored platelet group compared with fresh platelet group(p 〈 0.05), but was significantly lower than that in cold control group(p 〈 0.01). Although PagT(inducing reagent: C-PG) decreased, it could still be above 50% of fresh platelets. Survival time in rabbit vivo was close between UDP-Gal cold-stored platelet group and fresh platelet group(p 〈 0.05). Survival rate seventy-two hours after transfusion in fresh platelet group, UDP-Gal cold-stored platelet group and cold control group was 57.5%±7.2%,50.3%±6.3% and 0.1%±0.1% respectively. Rabbit ear bleeding time was significantly shortened after transfusion of galactosylation cooled rabbit platelet (p 〈 0.01), In contrast, it had less change in cold control group(p 〉 0.05). PPR was 66.1%±0.5%,47.8%±0.6%;60.9%±0.3%,41.6%±0.4%;47.7%±0.5%,9.4%±0.5% respectively in fresh platelet group, UDP-Gal cold-stored platelet group and cold control group. PPR after transfusion of galactosylation cooled rabbit platelet had no statistical difference compared with that of fresh platelet group(p 〉 0.05), and they in both groups were much higher than that in cold control group(p 〈 0.01). Conclusion: Galactosylation can improve functions of cooled rabbit platelets in vivo and in vitro. and prolong the storage time of them.

Type of Medium: Online Resource

ISSN: 0006-4971 , 1528-0020

URL: Article

DOI: 10.1182/blood.V108.11.3902.3902

RVK:

XA 33000

RVK:

XA 10000

Language: English

Publisher: American Society of Hematology

Publication Date: 2006

detail.hit.zdb_id: 1468538-3

detail.hit.zdb_id: 80069-7

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