The predominant role of the spleen in lymphocyte recirculation. I. Homing of lymphocytes to and release from the isolated perfused pig spleen.

Lymphocyte recirculation through the isolated pig spleen was studied by means of a perfusion system which kept the organ alive for a prolonged period of time. By changing the perfusate to a leucocyte-enriched or cell-free perfusate and taking serial arterial and venous samples, the numbers of lymphocytes which homed to or were released from the spleen were measured. In all experiments more lymphocytes homed than were released per minute. There was no apparent difference when autologous or allogeneic cells were used. The number of lymphocytes released depended on the number of lymphocytes homed previously. During the phase of constant release up to 3-3 X 10(6) lymphocytes were released per gram spleen per minute. From these values it can be extrapolated that up to 270 X 19(9) lymphocytes recirculate through the isolated pig spleen per day. Based on kinetic data from other species it is estimated that in the entire pig a total number of 300-400 X 10(9) lymphocytes recirculate per day. Thus, it can be concluded that the spleen is the most important organ for lymphocyte recirculation in the pig.     

THE KINETICS OF LYMPHOCYTE RECIRCULATION WITHIN THE RAT SPLEEN

The migration of lymphocytes from the blood into the splenic pulp and the release of lymphocytes from the spleen into the blood was studied by isolating the rat spleen and perfusing it with 15 ml of recirculating, oxygenated blood. When thoracic duct lymphocytes labelled with tritiated uridine were added to the initial perfusate the concentration of these cells fell exponentially for 2–3 hr and then rose to a flat secondary peak. From this pattern it was inferred that small lymphocytes entered the spleen at a rate proportional to their instantaneous concentration in the perfusate, traversed the splenic pulp and re-entered the perfusate with a minimum transit time of 2–3 hr. The rate of release of small lymphocytes from the spleen was not influenced by the prevailing concentration of small lymphocytes in the perfusate but probably reflected the rate of migration into the spleen over a period earlier than 2 hr before. The rate of exchange of small lymphocytes between the blood and the intact spleen in vivo was estimated to be about 84 × 10⁶ cells/hr. The size of the intrasplenic pool of recirculating small lymphocytes was probably 400–500 × 10⁶ cells. The rate of migration of small lymphocytes into the spleen was not affected by prior irradiation of the spleen donor. When either of two antigenic materials were added to the perfusate no inhibition of lymphocyte migration into the spleen was noted although the release of lymphocytes from the spleen was diminished by the addition of a large dose of sheep erythrocytes.     

Splenic lymphocytopoiesis and migration pattern of splenic lymphocytes

The spleens of young pigs were selectively labeled with tritiated thymidine ([³H]-TdR) and the relative and absolute numbers of labeled lymphocytes found 24 hr later in different lymphoid and nonlymphoid organs were determined autoradiographically. It was deduced that about 4.6 × 10⁹ lymphocytes (that is, about 15% of all splenic lymphocytes) are produced by the spleen per day and about 17% of the newly formed lymphocytes leave the spleen within the first day of labeling. Spleen-derived lymphocytes could be found in relatively high numbers in the lymph nodes, blood, gut-associated lymphoid tissues, and, surprisingly, in the bone marrow, whereas the concentration in the thymus was very low. In a second series, pigs were labeled with [³H]TdR and only the spleen was excluded from labeling. The labeling index of splenic small lymphocytes was about 10% 1 day later, indicating a high rate of influx of newly formed lymphocytes into the pig spleen. The spleen of the young pig is an important lymphocytopoietic organ and exports and imports newly formed lymphocytes at high rates.     

THE PREDOMINANT ROLE OF THE SPLEEN IN LYMPHOCYTE RECIRCULATION

Autologous blood lymphocytes from three normal pigs were labelled with ³H-uridine and retransfused before and after splenectomy. Frequent samples for up to 150 min after retransfusion were evaluated autoradiographically to determine the rate of disappearance of labelled lymphocytes from the blood. In one pig retransfusion was performed before and after sham-splenectomy. In all preoperative experiments the pattern of disappearance of labelled lymphocytes was very similar. After a first rapid decline (halving time on average 8 min) a short rise of the labelling index was observed from 10 to 15 min after retransfusion. Then a second more gradual decrease of labelled lymphocytes followed. The mean halving time during this period was less than 32 min. From 60 min onwards the labelling index remained nearly constant. Retransfusions performed 3 days after splenectomy revealed only one nearly constant decline of the labelling index (halving time on average 129 min). After sham-splenectomy the pattern of disappearance was similar to the preoperative experiment. One hour after the end of retransfusion the labelling index had decreased by three-quarters of the initial value in normal pigs and by only one-third in the splenectomized ones. These results indicate that in the pig the total rate of recirculation is at least 4 times faster with the spleen in situ than without the spleen.     

Alpha glucosidases in white blood cells, with reference to the detection of acid alpha 1-4 glucosidase deficiency.

The iron-containing violet acid phosphatases from beef spleen and pig allantoic fluid have been purified to homogeneity. Molecular weight determinations by zonal gel filtration, SDS-gel electrophoresis, and ultracentrifugation support values close to 40,000 for both enzymes, necessitating reappraisal of literature values. Similarly, the equivalent weight for iron is close to 20,000 for both enzymes, indicating the presence of two iron atoms per molecule of enzyme. The enzymes also have very similar ultraviolet and visible spectra, with λ_max values close to 550 nm, and ?₅₅₀ values(in terms of iron) of 2.04 × 10³ and 2.00 × 10³ for the beef spleen and pig allantoic fluid enzymes respectively.     

Kinetics of microtubule formation after cold disaggregation of the mitotic apparatus

The rate of spindle-fiber reformation following cold treatment of the giant amoeba, Chaos carolinensis, has been determined and used to test a single growth point, subunit incorporation model of microtubule assembly. Mitotic apparatuses isolated at one-minute intervals after rewarming contain progressively longer spindle fibers; re-assembly begins at the kinetochore region, proceeds at a rate of 1·5 μm per minute, then slows as the normal length of 5 μm is approached. From information on microtubule ultrastructure, the total number of 40-Å subunits in mitotic apparatuses per amoeba, and hence the concentration released during disassembly, was calculated to be 1·0 × 10¹⁵ molecules per cm³. Calculation of diffusion and assembly kinetics indicates that this concentration of microtubule subunits is equal to the concentration required to produce a growth rate of 1·5 μm per minute by diffusion of single subunits to one assembly point per microtubule.     

GRAFT SIZE CONSIDERATIONS IN THE KINETICS OF SPLEEN COLONY DEVELOPMENT

The kinetics of spleen colony development has been studied after the injection of 10⁶, 10⁵ and 3 × 10⁴ bone marrow cells. The results indicate that:

• 1 The CFU population growth rate is independent of cell dose until the logarithmic growth phase is passed. Slowing of growth was seen by day 12 after the highest dose, by day 15 after the median dose, but was not observed during the period of observation after the low dose.
• 2 The growth rate of CFU per colony is independent of cell dose, but the curves are not identical. The differences between the curves leads to the conclusion that there is a dose-dependent delay in the commencement of CFU proliferation. The delay is roughly equal to one cell cycle time between the medium and high inoculum groups and also between the medium and low inoculum groups.
• 3 The number of cells per colony is graft size dependent, the doubling times, where these can be roughly assessed, being inversely related to the graft size. From the average number of cells per colony on day 6 it is calculated that the mean doubling time in the early stages of colony development is less than 7 hr.
• 4 The proportion CFU:colony cells is dose dependent with the highest inoculum having the highest proportion and the low inoculum group having the lowest proportion.

     

The number of spermatozoa required by naturally mated ewes and the ability of rams to meet these requirements

The fertility of naturally mated ewes was compared with the number of spermatozoa deposited, and the number of times they were mated. The number of spermatozoa received was estimated from ejaculates flushed directly from the vagina of naturally mated ewes.In one experiment, maximum fertility was achieved with as few as 140 × 10⁶ spermatozoa. The percentage of pregnant ewes was similar in ewes mated once or more than once (68.4% vs. 72.5%). Similar results were obtained in one test of a further experiment but in a second test fertility was higher in ewes that were mated more than once. If this effect was due to the extra spermatozoa received, then ewes required 500 × 10⁶ spermatozoa to achieve maximum fertility. Half of the ewes were mated at their first oestrus after treatment with progestagens in the second experiment. The fertility of these ewes was similar to that of the remaining ewes, which were mated at natural oestrus.The mean number of spermatozoa ejaculated by individual rams varied from 140 × 10⁶ to 1050 × 10⁶, following depletion of the epididymal reserves of spermatozoa. The rams ejaculated an average of 9.1 × 10⁶ spermatozoa per gram of testis per day in the first experiment. The rams mated an average of 10.9 times per day in the first experiment, 6.9 and 6.1 times per day, respectively, for the first and second tests in the second experiment. The number of times that rams mated was highly correlated with the number of ewes with which they mated in the second experiment.     

Restoration of the Immune Response to Sheep Erythrocytes by a Serum Factor

THE immune response of CBA mice to sheep erythrocytes (SRBC) is known to be thymus-dependent because strain members thymectomized during the first few hours of life exhibit a marked inability to respond to this antigen^1,2. Experiments with isoantisera suggested that a cell to cell interaction is involved in this response. Thymus cells per se do not develop into haemolytic plaque-forming cells, but in some, so far obscure, way they cause cells of bone marrow origin to become producers of haemolytic plaques^2,3. A study of spleen cells from neonatally thymectomized (NNT) mice in a tissue culture system indicated that the decreased responsiveness to SRBC is also expressed in vitro. In that case 15×10⁶ NNT spleen cells produced only 500 haemolytic plaques when assayed on day 4 of culture. But when 15×10⁶ thymus cells were added to identical cultures of NNT spleen cells at inception, the number of haemolytic plaque forming cells increased to 2,300 (ref. 4). When an equivalent number of thymus cells alone were incubated with SRBC there was no response.     

Factors which may affect removal of protamine from sperm DNA during fertilization in the rabbit

In order to derive information about possible mechanisms by which the sperm head is converted into the male pronucleus during fertilization in the rabbit, unfertilized egg homogenate was assayed for two enzyme activities. Protamine was extracted from rabbit sperm, purified, and labelled with [¹⁴C] in an in vitro reaction and used as a probe to assay for a protein kinase which could transfer [³²P]PO₄ from [γ-³²P]ATP onto the substrate. A kinase with a pH optimum of approximately 8.0 to 8.5 is described. Assays for the enzyme glutathione reductase were performed using homogenates from eggs or embryos at three early stages of development. Results suggest that oocytes can oxidize 2.58 × 10^?6 μmol NADPH per minute per oocyte, unfertilized eggs 5.16 × 10^?7 μmol NADPH per minute per ovum, and 20- to 24-hour postcoitus fertilized eggs 2.30 × 10^?6 μmol NADPH per minute per ovum. The relevance of these observations to male pronuclear formation is discussed.     

The Effect of Manganese-induced Cytotoxicity on mRNA Expressions of HSP27, HSP40, HSP60, HSP70 and HSP90 in Chicken Spleen Lymphocytes in Vitro

The purpose of this study was to investigate the effect of manganese (Mn)-induced cytotoxicity on heat shock proteins in chicken spleen lymphocytes. Lymphocytes were cultured in medium in the absence and presence of MnCl₂ (2?×?10^?4, 4?×?10^?4, 6?×?10^?4, 8?×?10^?4, 10?×?10^?4, and 12?×?10^?4 mmol/L) for 12, 24, 36, and 48 h in vitro. Then, the mRNA levels of HSP27, HSP40, HSP60, HSP70, and HSP90 were examined by real-time quantitative PCR. The results showed that the mRNA levels of HSP27, HSP40, HSP60, HSP70, and HSP90 in all treatment groups at all time points, except mRNA levels of HSP27 at 48 h, had the same tendency. As manganese concentration increased, the mRNA expression of the heat shock proteins first increased and then decreased. In other words, we demonstrated that the mRNA expression of the heat shock proteins was induced at lower concentrations of manganese and was inhibited at higher concentrations. Mn had a dosage-dependent effect on HSP27, HSP40, HSP60, HSP70, and HSP90 mRNA expression in chicken spleen lymphocytes in vitro.     

DIFFERENCES IN THE NUCLEAR RIBONUCLEIC ACID CONTENT IN DIFFERENT AREAS OF THE HUMAN ADULT AND FOETAL BRAIN*

Abstract— Four different areas of ten brains from adults in the age group between 44 and 74 years and two areas of six foetal brains were studied. The cellular density was similar in the different areas of the brain of adult man; it averaged 11.9 × 10⁷/g wet tissue. The number of neurons per g wet tissue varied from 2.22 × 10⁷ in the cortex to 0.15 × 10⁷ in the centrum semiovale. In the brain of adults the overall RNA content of nuclei was higher for the cortex than for the corpus callosum or the centrum semiovale. The RNA content of neuronal nuclei was higher than that of non-neuronal nuclei. In the brain of foetuses the nuclear density was higher than in adults. The DNA content of a nucleus in foetal brain was 2–3 times as high as in adult brain and it approached adult values with increasing maturity.     

Mathematical Modeling Reveals Kinetics of Lymphocyte Recirculation in the Whole Organism

The kinetics of recirculation of naive lymphocytes in the body has important implications for the speed at which local infections are detected and controlled by immune responses. With a help of a novel mathematical model, we analyze experimental data on migration of ⁵¹Cr-labeled thoracic duct lymphocytes (TDLs) via major lymphoid and nonlymphoid tissues of rats in the absence of systemic antigenic stimulation. We show that at any point of time, 95% of lymphocytes in the blood travel via capillaries in the lung or sinusoids of the liver and only 5% migrate to secondary lymphoid tissues such as lymph nodes, Peyer''s patches, or the spleen. Interestingly, our analysis suggests that lymphocytes travel via lung capillaries and liver sinusoids at an extremely rapid rate with the average residence time in these tissues being less than 1 minute. The model also predicts a relatively short average residence time of TDLs in the spleen (2.5 hours) and a longer average residence time of TDLs in major lymph nodes and Peyer''s patches (10 hours). Surprisingly, we find that the average residence time of lymphocytes is similar in lymph nodes draining the skin (subcutaneous LNs) or the gut (mesenteric LNs) or in Peyer''s patches. Applying our model to an additional dataset on lymphocyte migration via resting and antigen-stimulated lymph nodes we find that enlargement of antigen-stimulated lymph nodes occurs mainly due to increased entrance rate of TDLs into the nodes and not due to decreased exit rate as has been suggested in some studies. Taken together, our analysis for the first time provides a comprehensive, systems view of recirculation kinetics of thoracic duct lymphocytes in the whole organism.     

ALGAL CELL DISRUPTION USING A PYREX TISSUE GRINDER AND THE B. BRAUN HOMOGENIZER1

A motor-driven Pyrex tissue grinder (PTG) and the B. Braun cell homogenizer (BH) were used to disrupt cells of Selenastrum capricornutum Printz for chlorophyll extraction. Cell disruption efficiency depended upon the number of cells filtered. Within the range of 2 × 10⁶ to 8–9 × 10⁶ algal cells per 2.4 cm filter, the PTG allowed more complete extractions. Beyond that number of cells, the BH was more efficient. The algal mass corresponding to 8–9 × 10⁶ cells was 0.14–0.17 mg dry weight.     

Laboratory culture and evaluation of the tubeworm Ficopomatus enigmaticus for biofouling studies

Ficopomatus enigmaticus, a euryhaline tube-building polychaete worm with a subtropical to temperate distribution, is an increasingly problematic fouling organism. In this study, laboratory protocols for maintaining adult broodstock, destructive spawning, larval culture and a settlement bioassay were developed. The method routinely yielded approximately 200 larvae per spawning adult. The mean number of eggs released by females was 1517 and the mean number of spermatozoids per male was 4.425?×?10⁶. Fertilisation success, using an initial concentration of 2.5?×?10⁶ spermatozoids and 45?eggs?ml^?1, was 76% after a contact time of 60?min. The first cleavage occurred after 20?min and the trocophore larval stage was attained by 18?h. Metatrochophores were observed 4?d post-fertilisation and were competent to settle 1?day later. The proportion of larvae that settled after 48?h was surface-dependent: 10.24% on glass, 1.39% on polystyrene and 11.07% on a poly(dimethylsiloxane) elastomer. The presence of a biofilm on glass increased the rate of settlement 7-fold compared to clean glass.     

Internal dose assessment of <Superscript>210</Superscript>Po using biokinetic modeling and urinary excretion measurement

The mysterious death of Mr. Alexander Litvinenko who was most possibly poisoned by Polonium-210 (²¹⁰Po) in November 2006 in London attracted the attention of the public to the kinetics, dosimetry and the risk of this high radiotoxic isotope in the human body. In the present paper, the urinary excretion of seven persons who were possibly exposed to traces of ²¹⁰Po was monitored. The values measured in the GSF Radioanalytical Laboratory are in the range of natural background concentration. To assess the effective dose received by those persons, the time-dependence of the organ equivalent dose and the effective dose after acute ingestion and inhalation of ²¹⁰Po were calculated using the biokinetic model for polonium (Po) recommended by the International Commission on Radiological Protection (ICRP) and the one recently published by Leggett and Eckerman (L&E). The daily urinary excretion to effective dose conversion factors for ingestion and inhalation were evaluated based on the ICRP and L&E models for members of the public. The ingestion (inhalation) effective dose per unit intake integrated over one day is 1.7 × 10⁻⁸ (1.4 × 10⁻⁷) Sv Bq⁻¹, 2.0 × 10⁻⁷ (9.6 × 10⁻⁷) Sv Bq⁻¹ over 10 days, 5.2 × 10⁻⁷ (2.0 × 10⁻⁶) Sv Bq⁻¹ over 30 days and 1.0 × 10⁻⁶ (3.0 × 10⁻⁶) Sv Bq⁻¹ over 100 days. The daily urinary excretions after acute ingestion (inhalation) of 1 Bq of ²¹⁰Po are 1.1 × 10⁻³ (1.0 × 10⁻⁴) on day 1, 2.0 × 10⁻³ (1.9 × 10⁻⁴) on day 10, 1.3 × 10⁻³ (1.7 × 10⁻⁴) on day 30 and 3.6 × 10⁻⁴ (8.3 × 10⁻⁵) Bq d⁻¹ on day 100, respectively. The resulting committed effective doses range from 2.1 × 10⁻³ to 1.7 × 10⁻² mSv by an assumption of ingestion and from 5.5 × 10⁻² to 4.5 × 10⁻¹ mSv by inhalation. For the case of Mr. Litvinenko, the mean organ absorbed dose as a function of time was calculated using both the above stated models. The red bone marrow, the kidneys and the liver were considered as the critical organs. Assuming a value of lethal absorbed dose of 5 Gy to the bone marrow, 6 Gy to the kidneys and 8 Gy to the liver, the amount of ²¹⁰Po which Mr. Litvinenko might have ingested is therefore estimated to range from 27 to 1,408 MBq, i.e 0.2–8.5 μg, depending on the modality of intake and on different assumptions about blood absorption.     

[3H]HARMALINE AS A SPECIFIC LIGAND OF MAO A–II. MEASUREMENT OF THE TURNOVER RATES OF MAO A DURING ONTOGENESIS IN THE RAT BRAIN

The combined measurement of MAO A activity (using [³H]5-HT as a specific substrate) and [³H]harmaline binding capacity indicated that the concentration of MAO A in brain was higher in 14-28 day old rats than in adult animals. The turnover rates of this enzyme in the forebrain and the brain stem of young (14-28 day old) and adult rats were calculated by following the recovery of MAO A activity and of [³H]harmaline binding capacity after an acute treatment with pargyline (75mg/kg i.p.). Both the fractional rate constant for MAO A degradation and its synthesis rate per g of fresh tissue were significantly higher in young animals. However, the calculation of the absolute synthesis rates of MAO A per brain area gave very similar values in young and adult animals: 1.3-1.5 × 10¹³ molecules of MAO A synthesized per day in the forebrain and 2.3-2.9 × 10¹² molecules per day in the brain stern. The results illustrate the validity of using [³H]harmaline binding to evaluate possible changes in the turnover rate of MAO A in tissues.     

Mitogen-induced T-lymphocyte proliferation: a reappraisal of the early requirement of extracellular ionized calcium.

Mitogen-induced DNA synthesis in lymphocyte cultures requires an extracellular calcium concentration of 3 × 10^?6M or higher. When cultures of human or mouse lymphocytes were incubated with T-cell mitogens for the first 12 hours in a medium with about 3 × 10^?6M calcium ion concentration, and then the normal calcium concentration was restored, the induction of DNA synthesis in the cultures was salvaged, but it started 10–16 hours later than in control cultures. Lipopolysaccharide-induced thymidine incorporation in mouse spleen cell cultures responded to this experimental design in a more complex way. - These results support the idea that calcium ions are specifically needed for one or more of the very early steps in mitogenic activation of T-lymphocytes.     

Electron microscopy of human interphase nuclei

Quantitative electron microscopy was used to analyze surface-spread, critical-point-dried human interphase nuclei and chromatin. The following information is presented: (1) Unstimulated interphase nuclei of lymphocytes from peripheral blood have a mean dry mass of 50.30×10^?12 g. The mean dry mass of stimulated nuclei of lymphocytes was determined to be 59.34×10^?12 g, a significant statistical difference from the unstimulated ones. (2) Mean diameter of chromatin fibers and mean fiber mass per micron were 199ű15% coefficient of variation (C.V.) and 5.95×10^?16g×29% C.V., respectively. (3) A line of regression of fiber mass on fiber diameter for 83 fibers indicated that a 200-Å fiber has a mass of 5.86×10^?16g/μ, or almost the same as the mean fiber mass of 5.95× 10^?16g/μ. (4) With the value 7×10^?12g for the DNA content of an unstimulated lymphocyte nucleus, a total length of 215 cm is calculated for the DNA double helix. When this length is compared to the mean length of chromatin fiber per nucleus (7.59 cm), a ratio of 28.3 to 1 results, which is called the DNA-packing ratio. (5) This DNA-packing ratio of 28.3 is reasonably close to the packing ratio of 26.9 suggested from model calculations for the second DNA supercoil in a 200-Å chromatin fiber.     

Formation of heterophile antibodies by human tonsilar lymphocytes: II. In vitro stimulation with allogeneic cells

Short-term cultures of human tonsilar lymphocytes (HTL), 5 × 10⁶ cells/culture, in medium RPMI 1640 supplemented with human group AB serum were studied for the production of plaque-forming cells (PFC) against sheep (SRBC) and bovine (BRBC) red blood cells following in vitro stimulation by various allogeneic lymphoid cells. Of 55 HTL specimens examined, 48 produced a significant number (50–300/culture) of PFC against SRBC and/or BRBC following the in vitro stimulation. The optimal doses of the stimulator HTL and peripheral blood lymphocytes (PBL) were 10⁷ and 5 × 10⁶/culture, respectively. After the stimulation, PFC appeared in significant numbers on the third day, reached the peak number on the sixth day, and decreased sharply in number thereafter. Removal of E-rosetting cells from both stimulator and responder populations abolished the PFC formation. PFC formation against SRBC was inhibited by solubilized Forssman antigen, while PFC formation against BRBC was inhibited strongly by Hanganutziu-Deicher antigen, hardly by Paul-Bunnell antigen and not at all by Forssman antigen. Supernatants of mixed lymphocyte culture of PBL were shown to enhance PFC formation of HTL cultures stimulated by allogeneic lymphocytes. The results of this study indicated that in vivo primed B cells of the HTL were triggered in vitro by allogeneic stimulation for the heterophile antibody formation. Since these antibodies are apparently directed against Forssman and Hanganutziu-Deicher antigens, the “allo” nature of these antigens as well as their relationship to the previously described heterophile transplantation antigens have to be clarified.