The Behavior, as Regards Shape and Volume, of Human Red Cell Ghosts in Fresh and in Stored Blood

Abstract (1) When human red cells are hemolyzed in very hypotonic media (NaCl of a tonicity of 0.167) and when the tonicity is restored, by adding appropriate amounts of NaCl, to tonicities such as 0.3, 0.5, 1.0, and 1.7, the mean volume of the ghosts appears to be linear with the reciprocal of the tonicity. This might lead one to conclude that the ghosts are osmometers and that their volume is governed by simple osmotic considerations such as those expressed by a modified van’t Hoff-Mariotte law. Examination of the shapes and volumes of individual ghosts by a technic which combines phase optics, electronic flash (exposure time 0.001 second) and photography shows that three distinct populations of ghost coexist in any tonicity. These are spherical ghosts with a mean volume of 150 µ3, discoidal biconcave ghosts with a mean volume of 85 µ3, and crenated ghosts with a smaller volume which can be calculated. The most likely reason for this complexity is that the shape and volume of the ghost depends partly on its structure, and not altogether on the tonicity of the surrounding medium. Simple osmotic laws have no real application to systems of this kind. (2) The changes in ghost volume and shape, as they depend on the duration of storage of the blood, at 4 C, from which the ghosts are prepared, and as they reflect changes in ghost structure, can be expressed simply. Crenated and discoidal ghosts certainly have some of the elements of red cell structure; the spherical ghost, which soon fragments and gives rise to myelin forms, may also retain some of the original elements of structure, but the fragment and the myelin form have certainly lost them. The latter objects are so small and light that they are not thrown down into the ghost column in the hematocrit tube, and so, as ghost structure disappears with increasing time of storage of the red cells from which they are prepared, a discrepancy appears between the volume of the ghost column as measured by the hematocrit and the volume which one would expect. This discrepancy can be used as a measure of the extent to which ghost structure is lost, and there comes a time, as the duration of red cell storage is increased, when the ghosts prepared from these red cells begin to be replaced by breakdown products such as myelin forms, etc. (3) The less the efficiency of the conditions of red cell preservation, the shorter is this time. In human blood rendered incoagulable with heparin, structural breakdown in the preceding sense and measured by a simple expression which changes sign when the loss of structure has reached a certain point, occurs after about 26 days. In human blood preserved in ACD, structural breakdown measured in an identical manner occurs after about 55 to 60 days. In human blood preserved in ACD-inosine, structural breakdown does not occur until about 75 to 80 days. These results are based on a large amount of preliminary work of an exploratory nature and then on three runs with heparin, five runs with ACD and five runs with ACD-Inosine.

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A Red Cell Enzyme Method for the Diagnosis of Acute Intermittent Porphyria

Blood ◽

10.1182/blood.v44.6.857.857 ◽

1974 ◽

Vol 44 (6) ◽

pp. 857-868 ◽

Cited By ~ 79

Author(s):

C. Richard Magnussen ◽

Joel B. Levine ◽

Joyce M. Doherty ◽

Judy O. Cheesman ◽

Donald P. Tschudy

Keyword(s):

Aminolevulinic Acid ◽

Acute Intermittent Porphyria ◽

Mean Value ◽

Red Cells ◽

Red Cell ◽

Enzyme Preparations ◽

Cell Enzyme ◽

Enzyme Method ◽

Latent Disease ◽

The Mean

Abstract A method has been devised for the measurement of uroporphyrinogen I synthetase ih red cells. By using trichloroacetic acid as a protein precipitant, heme is removed from the final solution, allowing accurate measurement of porphyrins. The method is highly reproducible and adaptable to varying incubation volumes and enzyme preparations. It is of great value as an enzyme diagnostic method for acute intermittent porphyria and appears capable of detecting patients with the latent disease who have normal urinary δ-aminolevulinic acid and porphobilinogen excretion. It also appears to distinguish other types of porphyria from acute intermittent porphyria. The mean value of the enzyme in red cells of patients with acute intermittent porphyria was approximately 50% that of normals, indicating that the mutation causes complete lack of catalytic activity in the mutant enzyme.

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Red cell permeability effect on the mean transit of an indicator transported through an organ by red cells and plasma.

Circulation Research ◽

10.1161/01.res.36.2.352 ◽

1975 ◽

Vol 36 (2) ◽

pp. 352-357 ◽

Cited By ~ 8

Author(s):

W Perl

Keyword(s):

Red Cells ◽

Cell Permeability ◽

Red Cell ◽

The Mean

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PACKED RED CELL DENGAN DELTA Hb DAN JUMLAH ERITROSIT ANEMIA PENYAKIT KRONIS (Packed Red Cells with Delta Hb and Erythrocytes in Anemia of Chronic Disease)

INDONESIAN JOURNAL OF CLINICAL PATHOLOGY AND MEDICAL LABORATORY ◽

10.24293/ijcpml.v21i3.1270 ◽

2018 ◽

Vol 21 (3) ◽

pp. 220

Author(s):

Novita Indayanie ◽

Banundari Rachmawati

Keyword(s):

Chronic Disease ◽

Iron Deficiency ◽

Iron Deficiency Anemia ◽

Strong Correlation ◽

Red Cells ◽

Deficiency Anemia ◽

Red Cell ◽

Anemia Of Chronic Disease ◽

Common Cause ◽

The Mean

Anemia chronic disease is the second common cause after iron deficiency anemia with hemoglobin levels below the referencevalue. The pathogenesis of anemia should be determined for treatment. Hematinics and or erythropoietin are other treatments besidestransfusion. The transfusion is started when Hb≤7g/dL. The PRC transfusion of 4ml/kg could increase Hb level by 1 g/dL, or 1 unit andcould increase 3–5% of hematocrit. The objective of this study was to know the correlation of PRC unit with delta Hb and erythrocytesin anemia of chronic disease. The 60 samples examined were from patients of the Kariadi Hospital Semarang suffering from anemia ofchronic disease and who were transfused with PRC from January up to March 2014. The study subjects comprised 28 men (46.7%) and32 women (53.3%), with a mean age of 47 years. The number of PRC given was between one (1) to four (4) units. The mean delta Hbwas 3.48 and the mean delta erythrocytes was about 1.03 (0.1 to 2.3). There was a significant correlation between PRC units and deltaHb (r:0.856, p:0.000), as well as delta erythrocytes (r:0.716, p:0.000). Based on this study, it can be concluded that PRC units have avery strong correlation with delta Hb and as well as with delta erythrocytes in patients suffering from anemia of chronic disease

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Nitrite and Red Cell Function in Carp: Control Factors for Nitrite Entry, Membrane Potassium Ion Permeation, Oxygen Affinity and Methaemoglobin Formation

Journal of Experimental Biology ◽

10.1242/jeb.152.1.149 ◽

1990 ◽

Vol 152 (1) ◽

pp. 149-166 ◽

Cited By ~ 2

Author(s):

FRANK B. JENSEN

Keyword(s):

Cell Function ◽

Oxygen Affinity ◽

Red Cells ◽

Red Cell ◽

In Vitro Experiments ◽

K Uptake ◽

The Mean ◽

K Release

Red cell function was studied in carp by a combination of in vivo and in vitro experiments with nitrite as the perturbing agent. In vivo accumulation of nitrite caused a marked increase in the red cell methaemoglobin content, and reduced the mean cellular volume. The oxygen affinity of unoxidized haemoglobin was strongly decreased, partly as result of the elevated concentration of cellular nucleoside triphosphates and haemoglobin associated with red cell shrinkage. Red cell pH was unchanged compared to controls, but reduced when referred to constant extracellular pH and O2 saturation. The mean cellular K+ content decreased, reflecting a K+ loss from the red cells during their shrinkage. This K+ loss contributed significantly to the large plasma hyperkalaemia during nitrite exposure. In vitro experiments revealed that nitrite influx into deoxygenated red cells was much larger than into oxygenated red cells. Nitrite permeation of the red cell membrane was not inhibited by DIDS and did not change extracellular pH. Methaemoglobin (MetHb) formation was more pronounced in deoxygenated blood than in oxygenated blood, but quasi-steady states were reached, reflecting a balance between nitrite-induced MetHb formation and the action of MetHb reductase. Red cells incubated in the oxygenated state released K+, whereas a net K+ uptake occurred in deoxygenated cells. Nitrite did not change the K+ loss from oxygenated cells, but shifted the K+ uptake in deoxygenated cells to a pronounced K+ release by the time high MetHb levels were reached. Both types of red cell K+ release were inhibited by DIDS and appeared to occur via a route involving Band 3. The data are consistent with the hypothesis that a significant DIDS-sensitive K+ efflux from the red cells occurs whenever a large fraction of the haemoglobin molecules assumes an R-like quaternary structure.

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Evolution of GPI-Deficient Clones Predicts Clinical Course in Paroxysmal Nocturnal Haemoglobinuria.

Blood ◽

10.1182/blood.v104.11.172.172 ◽

2004 ◽

Vol 104 (11) ◽

pp. 172-172 ◽

Cited By ~ 5

Author(s):

Stephen J. Richards ◽

Matthew J. Cullen ◽

Anita J. Dickinson ◽

Claire Hall ◽

Anita Hill ◽

...

Keyword(s):

Aplastic Anemia ◽

Clinical Course ◽

Spontaneous Remission ◽

Red Cells ◽

Red Cell ◽

Clone Size ◽

Clinical Behavior ◽

The Mean ◽

Pnh Clone

Abstract Flow cytometric analysis of GPI-linked antigens has had a major impact on the diagnosis of PNH. Significant numbers of patients with aplastic anemia have small PNH clones, and due to the precision in clone size measurement, reliable serial monitoring can now be undertaken although the clinical value of this is not proven. From our series of 234 PNH patients, we analysed clinical correlates between disease type and red cell and granulocyte peripheral blood clone sizes as determined by flow cytometry at presentation. For hemolytic patients (n = 99) the mean PNH clone sizes were: granulocytes 84.8%; red cells 45.3% (type III cells 33.6%). For aplastic patients (no macroscopic hemolysis) the mean clone sizes were: granulocytes 18.5%; red cells 6.4% (type III cells 4.5%). The two groups were statistically different (Mann Whitney U; P<0.001). Monitoring of PNH clones in 86 of these patients who had at least 3 samples over a minimum of 12 months (mean 55 months; range 15–174) not only showed distinct groups of patients with highly characteristic patterns of disease but also provided insights into the incidence of spontaneous remission, progression from aplastic to hemolytic disease, and development of leukemia. Firstly, hemolytic patients that present with >90% granulocyte clones (n = 30; mean follow up 48 months) with virtually all their hematopoiesis maintained from PNH stem cells have clone sizes that remain stable and their clinical behavior suggests that their PNH can persist for up to 40 years. The second group of patients (n = 16) were those with hemolytic PNH with granulocyte clones of <90%. Mean granulocyte clone size at presentation was 68.4% (range 34.7– 90%) with a mean follow-up of 66 months (range 24–164). Of these, 6 showed stable clone sizes, 2 increasing clone size, and 8 showing reductions in granulocyte clone size. The third group were those presenting with aplastic anemia (n = 34). This group showed the most significant variation in clone size and clinical behavior. Of the 12 patients with persistent aplastic anemia, the majority had slowly increasing clone sizes with 5 patients progressing to hemolytic PNH after a variable time period ranging from 26 to 79 months. Only 3 patients developed MDS or AML. Two of these were from the >90% granulocyte clone group (2/30) and developed as a terminal event, one with GPI-MDS, and the second with a rapid emergence of GPI+MDS. One patient in the aplastic group showed progression to AML (1/34). 27% of patients had an improvement in cytopenias with concurrent decrease in PNH clone size. For hemolytic patients with granulocyte clones of <90%, the 8 patients with falling clone sizes had improving blood counts. The PNH granulocyte clone halved in a mean of 74 months. Of the patients with aplastic anemia, 15 showed resolution of anemia with normalization of counts and all but one had an associated fall in granulocyte PNH clone sizes. Eleven patients have been treated in clinical trials of the anti-complement antibody, eculizumab, for a period of up to 2 years and over this period the proportion of PNH granulocytes has remained stable. This data demonstrates that the size and type of granulocyte and red cell PNH clones at presentation predicts the clinical course for individual patients assisting long term clinical management planning. Moreover, regular clone size monitoring predicts the likelihood of spontaneous reduction in the PNH clone and potentially for spontaneous remission.

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Erythrocyte alterations endurance exercise in horses

Journal of Applied Physiology ◽

10.1152/jappl.1981.51.1.131 ◽

1981 ◽

Vol 51 (1) ◽

pp. 131-134 ◽

Cited By ~ 31

Author(s):

J. H. Boucher ◽

E. W. Ferguson ◽

C. L. Wilhelmsen ◽

N. Statham ◽

R. R. McMeekin

Keyword(s):

Red Blood Cells ◽

Endurance Exercise ◽

Blood Cells ◽

Prolonged Exercise ◽

Red Cells ◽

Erythrocyte Count ◽

Red Cell ◽

Red Cell Indices ◽

The Mean

The erythrocytes of 14 conditioned horses participating in a 157-km endurance ride (requiring 14–21 h) were examined before the ride, immediately upon entering the 44–91-, and 130-km rest stops, and at the finish. At the first rest stop (44 km), the mean erythrocyte count increased 41% (P less than 0.001), the mean hematocrit (Hct) increased 30% (P less than 0.001) and the mean hemoglobin (Hb) increased 33% ( P less than 0.001). Although subsequent mean erythrocyte counts, Hct, and Hb values remained significantly elevated above controls, the values decreased 9–9% from the 4-km values later in the ride. These changes suggest a lost of red cells mass during the prolonged exercise. Spiculated red blood cells that increased markedly in number during exercise were also observed in these conditioned horses. The appearance of an increased number of spiculated red cells with exercise was associated with corresponding changes in red cell indices.

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Lactate and pyruvate gradients between red blood cells and plasma during acute asphyxia

Journal of Applied Physiology ◽

10.1152/jappl.1964.19.6.1100 ◽

1964 ◽

Vol 19 (6) ◽

pp. 1100-1104 ◽

Cited By ~ 22

Author(s):

Salha S. Daniel ◽

Hisayo O. Morishima ◽

L. Stanley James ◽

Karlis Adamsons

Keyword(s):

Sodium Lactate ◽

Red Cells ◽

Red Cell ◽

Cell Ratio ◽

Lactate And Pyruvate ◽

The Mean ◽

Endogenous Release ◽

Pyruvate Ratio

The rate of equilibration of lactate and pyruvate between plasma and red cells has been studied during asphyxia and following addition of sodium lactate in vivo and in vitro. In the resting, well-oxygenated guinea pig, the mean plasma/red cell ratio of lactate was 1.55 and that of pyruvate 2.47. During asphyxia, the plasma/red cell ratio of lactate rose and that of pyruvate fell, indicating a delay in equilibration. Incomplete equilibration affected particularly the lactate/pyruvate ratio in the two compartments. Infused neutral sodium lactate penetrated the red cells at a rate comparable to that observed following endogenous release of lactic acid during acute asphyxia. In vitro at pH 6.8@#X2013;7.4 at 38 C, the time to 50% equilibration of lactate between plasma and cells of human blood was less than 2 min. It is concluded that during acute asphyxia and resuscitation whole blood values of lactate and pyruvate do not bear a constant relationship to those of plasma. lactate/pyruvate ratio Submitted on March 16, 1964

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Red blood cell life span in the ovine fetus

AJP Regulatory Integrative and Comparative Physiology ◽

10.1152/ajpregu.2000.279.4.r1196 ◽

2000 ◽

Vol 279 (4) ◽

pp. R1196-R1204 ◽

Cited By ~ 22

Author(s):

Robert A. Brace ◽

Christiane Langendörfer ◽

Tae-Bok Song ◽

Donald M. Mock

Keyword(s):

Blood Cell ◽

Life Span ◽

Parameter Optimization ◽

Fetal Growth ◽

Red Blood Cell ◽

Red Cells ◽

Red Cell ◽

Fetal Circulation ◽

Cell Life ◽

The Mean

Red cell life span within the fetal circulation has not been reported, although erythrocyte life span has been studied in the adult and newborn. The present study quantified red cell life span in 12 chronically catheterized fetal sheep at 97–136 days gestation (term = 150 days) with the use of autologous red cells labeled with [14C]cyanate. Cyanate forms a permanent covalent bond with hemoglobin and acts as a permanent red cell label. In the fetuses, blood 14C activity decreased in a curvilinear fashion with time and reached 50% of the initial activity at 16.4 ± 1.6 (SE) days. In contrast, 14C activity of autologous red cells in two adult ewes decreased linearly with time as expected, reached 50% of the initial 14C activity in 59 days, and yielded life spans of 117 and 121 days. Computer modeling and parameter optimization taking into account growth and skewed life span distribution were used to analyze the 14C disappearance curve in each fetus. The mean life span of all red cells in the fetal circulation was 63.6 ± 5.8 days. Mean red cell life span increased linearly from 35 to 107 days as fetal age increased from 97 to 136 days ( r = 0.83, P < 0.001). Life span of cells produced at the time of labeling was significantly greater than the mean life span. Fetal growth rate estimated from parameter optimization was 3.28 ± 0.72%/day; this compared well with the rate of 3.40 ± 0.14%/day calculated from fetal weights at autopsy. Mean corpuscular volume decreased as a function of gestational age, but the decrease was small compared with the large increase in red cell life span. We conclude the following: 1) red cell life span in the fetal circulation is short compared with the adult; 2) red cells in younger fetuses have shorter life spans than in near-term fetuses; 3) the curvilinear disappearance of labeled red cells in the fetus appears to be due primarily to an expanding blood volume with fetal growth; and 4) red blood cell life span in a growing organism will be significantly underestimated unless the expansion of blood volume with growth is taken into account.

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STUDIES ON COPPER METABOLISM. XIX

Journal of Experimental Medicine ◽

10.1084/jem.103.5.701 ◽

1956 ◽

Vol 103 (5) ◽

pp. 701-712 ◽

Cited By ~ 38

Author(s):

J. A. Bush ◽

W. N. Jensen ◽

J. W. Athens ◽

Helen Ashenbrucker ◽

G. E. Cartwright ◽

...

Keyword(s):

Life Span ◽

Half Life ◽

Turnover Rate ◽

Copper Metabolism ◽

Red Cells ◽

Deficiency Anemia ◽

Red Cell ◽

Cell Life ◽

Iron Deficient ◽

The Mean

Ferrokinetic studies were performed in three copper-deficient swine and the results have been compared with similar studies in 18 normal pigs. The mean value for the plasma iron turnover rate in the deficient swine was 1.76 mg./kg. day; for the red cell iron incorporation rate, 1.24 mg./kg. day; for the red cell iron turnover rate, 1.18 mg./kg. day; for the red cell life span, 13 days. Corresponding figures in the normal swine were 1.11 mg./kg. day, 1.01 mg./kg. day, 0.59 mg./kg. day and 63 days, respectively. The red cell life span was measured by the use of radioactive chromium in a total of 26 pigs. The mean erythrocyte half-life of normal cells transfused into normal pigs was 17 days. The mean half-life of erythrocytes from copperdeficient swine transfused into copper-deficient swine was 9 days. The mean half-life of red cells from control animals transfused into copper-deficient swine was 16 days while that of erythrocytes from copper-deficient swine transfused into normal pigs, was 13 days. The mean half-life of cells from iron-deficient pigs transfused into iron-deficient pigs was 19 days. It is concluded that copper deficiency anemia results from both a shortened erythrocyte survival time and limited capacity of the bone marrow to produce red cells. It is suggested that copper is an essential component of erythrocytes in swine.

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QUANTITATIVE ASPECTS OF THE RED BLOOD CELL AGGLUTINATION TEST FOR INFLUENZA VIRUS

Journal of Experimental Medicine ◽

10.1084/jem.79.2.185 ◽

1944 ◽

Vol 79 (2) ◽

pp. 185-195 ◽

Cited By ~ 52

Author(s):

Gail Lorenz Miller ◽

W. M. Stanley

Keyword(s):

Influenza Virus ◽

Agglutination Test ◽

Red Cells ◽

Unit Weight ◽

Red Cell ◽

Cell Agglutination ◽

Quantitative Measurements ◽

Chemical Purity ◽

Method Of Measurement ◽

The Mean

A detailed study has been made of the nature of the variables inherent in the chicken red cell agglutination test for influenza virus in an effort to obtain a method of measurement of biological activity of sufficient accuracy that it might be employed as a reliable index of chemical purity of preparations of the virus. It was found that the temperature at which the test is conducted has a marked effect on the titer, whereas within the range of pH 6–8 the pH has a negligible effect. It was also found that a variation in results may be encountered due to a variation in the specific behavior of red cells from different chickens and to an instability of the red cells themselves. Preparations of purified influenza virus held at 4°C., on the other hand, were found to be stable with respect to chicken red cell agglutinating activity for several months. This fact, together with the fact that in duplicate measurements upon different samples the accuracy was such that the chances were 19 out of 20 that differences of 8.4 per cent in the mean end points were significant, made it possible to establish a reproducible standard of CCA activity based on a unit weight of purified virus material. As a result, it was possible to devise a standardized procedure for carrying out with high accuracy quantitative measurements of influenza virus.

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