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As a link in a series of studies on the effects of blood constituents on the brain function by means of brain perfusion, we used four kinds of artificial blood; namely, the blood containing a low molecular dextran, one containing glutamic acid, one containing essential amino acid group and the one containing both essential amino acid group and glutamic acid. During the perfusion experiments we observed the effects of blood constituents on the function and metabolism of the perfused brain and obtained the following results. 1. When a low molecular dextran is used as the colloid osmotic pressure agent instead of hydrodextran, the amount of the blood flow in the brain is maintained roughly at a certain fixed level throughout the experiment, showing no gradual decreasing tendency. 2. When using the artificial blood supplemented with glutamic acid, EEG of the perfused brain shows an increase in the appearance rate of β32 and β33 bands, approaching closely to the pattern of EEG of unrestrained controls at arousal state. 3. In the case of the blood added with essential amino acids similar to the case using the blood with glutamic acid, EEG approaches towards the alert pattern of the controls. 4. When the perfusion is done with the artificial blood lacking in amino acids, about one hour after the start of the perfusion the amount of glutamic acid and its related compounds in the brain can no longer be maintained at normal level and the decrease, being so marked, brings about a marked decrease also in total amino acid content. 5. When the perfusion blood contains glutamic acid, essential amino acid group or both, the concentrations of amino acids of the brain glutamic acid group and the total amino acid can be maintained approximately at normal level for the duration of over one hour.

An electron microscopic study on the fine structural differences of motor endplates among the red, white and intermediate muscle fibers of the rat intercostal muscles was made and the following results were obtained. 1. In the motor endplate of the red fiber, the junctional folds were poorly developed and their number was small. 2. In the motor endplate of the white fiber, the junctional folds were well developed and their number was far more numerous than those in the red fiber. 3. The fine structure of the motor endplate of the intermediate fiber was of an intermediate character between the red and white fiber.

Since Hahn's observation of the postalimentary lipemia clearing actIvity following the injection of heparin, physiological, biochemical and clinical significances of the postheparin lipoprotein lipase have been well clarified. The presence of the endogenous lipoprotein lipase in human blood, which was at first doubted, has been repeatedly confirmed2∼8. Recent papers9,10 described elevated endogenous lipoprotein lipase activity in patients with essential hyperlipemia after ample fat uptake. In this preliminary report, changes of the lipoprotein lipase activity during oral glucose tolerance test is illustrated.

1. An oligomycin -sensitive ATPase was isolated and partially purified from beef heart mitochondria. The specific activity of ATPase sensitive to oligomycin of the fraction was five to eight times that of aged mitochondrial or of DNP-induced mitochondrial ATPase assayed under the same condition. 2. Electron micrographs of the partially purified oligomycin- sensitive ATPase reveal a structure in which headpieces are regularly attached by way of stalks to a thread-like structure derived from a superficial portion of base pieces. 3. A high concentration of the structured material coincided with a high activity of oligomycin-sensitive ATPase. When the headpieces were detached from the structure, the ATPase became insensitive to oligomycin. 4. The fraction of oligomycin -sensitive ATPase was essentially free of membrane structure and was contaminated with a small amount of cytochromes b and Cl but no cyt. a. Cytochrome concentrations of the preparations were indifferent to the activity of oligomycin sensitive ATPase. It follows that ATPase does not require cytochromes or membrane structure for its oligomycin sensitivity. 5. From these results it seems that the factor rendering ATPase sensitive to oligomycin should be contained in the stalks and/or the thread-like portion of basepieces of the structure. The structure is the simplest unit of oligomycinsensitive ATPase as yet obtained. 6. The structure was called "oligomycin-sensitive ATPase particles" (abbreviated as OSA particles). A unit of OSA particles consists of a headpiece attached by a stalk to a portion of base piece.

The site of localization of TCA cycle dehydrogenases in mitochondria has been investigated by observing the dehydrogenase activities and fine structure of the fractionated samples after freezing and thawing or sonication of beef heart and rat liver mitochondria. 1. In the sonicated mitochondria, activities of malic and isocitric dehydrogenases were highest in the supernatant fraction centrifuged at 198,000 x g for 60 minutes, while the specific activity of a-ketoglutaric dehydrogenase was higher in the fluffy or residue fraction. The distribution of the activity of pyruvic dehydrogenase was similar to that of a-ketoglutaric dehydrogenase. 2. In a sucrose density gradient fractionation of the fluffy fraction obtained by centifugation of sonicated mitochondria at 198, 000 x g for 60 minutes, the activities of malic and pyruvic dehydrogenase were observed in the top (or low density) layer in the form of fine particles, while that of a-ketoglutaric dehydrogenase was observed in the middle (or medium density) layers in the form of aggregates of fine particles and membranous fragments. 3. In the samples fractionated after freezing and thawing of mitochondria, which were considered to be a relatively mild disruption, the specific activity of a-ketoglutaric dehydrogenase was higher in the residue (submitochondria) fraction than that in the supernatant fraction (centrifuged at 144,000 x g, 30 minutes), and the activity of malic dehydrogenase still remained significantly high in the residue fraction. 4. It was deduced that the TCA cycle dehydrogenases could be localized in the matrix of the mitochondria by a loose binding to the inner membrane.

The results of our study may briefly be summarized as follows: 1) The irradiation with microrays (20∼30 watts) similar as 2,000 R and 5,000 R Gamma radiation did not substantially affect the activity of fibrinolysin (SK+SD). 2) By the irradiation method so far mentioned it has been demonstrated that the fibrinolytic activity of anticoagulant of the SK+SD preparation is preserved in all the clotting systems which we used. 3) Our findings indicate that it is possible to irradiate patients for therapeutical purpose with Radarmed (electromagneticrays) provided that there is produced some enhancing influence of the same blood clotting factors or systems. Together with earlier works in this field it appears that this method of the microirradiation could provide us with an important evidence on which we can base our further in vitro and in vivo radiohematologic studies; investigations with various preparations, types of radiation that are still underway9∼16.

With a certain fixed methods of analyses, we carried out the determination of flavins and cytochromes in the mitochondria (Mt) and electron transfer particles (ETP) of the heart and liver of rats and cows, and made a comparison of the data with one another. Our findings may briefly be summarized as follows. 1. The concentration of each component of the beef heart mitochondria proved to be 0.47 for acid extractable flavins; 0.22 for acid nonextractable flavin; O. 75 for cytochrome (cyt.) a; 0.58 for cyt. b; and O. 51 for cyt. C + Cl, all units being mμ mole per mg of protein. 2. In the beef liver mitochondria it was 0.46 for acid extractable flavins; 0.18 for acid non-extractable flavin; 0.092 for cyt. a; 0.089 for cyt. b; and 0.122 for cyt. C+Cll likewise all units in term of mμ mole per mg of protein. 3. In the case of rat heart mitochondria, it was found to be O. 42 for acid extractable flavins; 0.22 for acid non-extractable flavin; 0.88 for cyt. a; 0.41 for cyt. b; and 0.62 for cyt. C + Cll all in mμ mole per mg of protein. 4. In the rat liver mitochondria it was 0.56 for acid extractable flavins; 0.19 for acid non-extractable flavin; 0.20 for cyt. a; 0.14 for cyt. b; and 0.19 for cyt. C+Cl. 5. The concentration ratios of Fs, cyt. a and cyt. b of the mitochondria, what are considered to be intrinsic and fixed components of the mitochondrion. to those of the electron transfer particles were 1. 3 in both the beef heart and the rat heart, while 2.2 in the beef liver and 2.1 in the rat liver. 6. These findings were compared with the data reported by other workers, and also a discussion was made on the molecular organization of the mitochondrial inner membrane.

For the purpose to know whether the annual increase of leukemia incidence in Japan is due to some leukemogenic factors or due to the increased detection rate, the authors made some statistical survey of autopsy cases in which the diagnosis is reliable and not any type of leukemias escape the detection. The results showed that acute leukemias, which are found mostly in younger age, is actually increasing. In addition, it has been deduced that among the suspected factors the increase in ionizing radiation will be one of the most probable factors for the increase in leukemia incidence

In order to know the precise quantity of catalase protein in acatalasemic and hypocatalasemic blood, immunological studies were conducted using hemolysates or acetone extracts of those blood as antigen. 1) The ratio of catalase contained in normal, hypocatalasemic and acatalasemic blood, calculated from precipitates produced in the reaction between catalase antibody and hemolysates was 1.0 : 0.5 : 0.07. 2) The ratio of catalase in normal, hypocatalasemic and acatalasemic blood, calculated from precipitates from the catalase antibody and the acetone extracts was 1.0: 0.49 : 0.11. In the precipitin ring tests using acetone extract, the antigen titer in normal, hypocatalasemic and acatalasemic extracts was 40, 20, and 0 respectively. 3) From our experiments it can be said that hypocatalasemic blood shows one half the catalase activity of normal blood, due to one half the quantity of catalase protein, and that acatalasemic blood lacks catalase activity due to the absence of the catalase protein. These findings strongly suggest that no substances exist which suppress or inhibit the catalase activity in hypocatalasemic and acatalasemic blood.

Bei 365 Leberpatienten wurde die BTS im Blut bestimmt und bei einem Teil der Fälle wurde die Leberkatheterisation durchgefiihrt. Das fiihrte zu folgenden Ergebnissen : 1) Der BTS-Blutspiegel war ungefähr in 50 Prozent der Fälle erh&#öht, und zwar fallend in der Reihenfolge bei Leberzirrhose, akuter Hepatitis und chronischer Hepatitis. Bei der akuten Hepatitis war er in der Rekonvaleszenz erhöhter als im akuten Stadium und auch bei chronischer Hepatitis war er bei längerem Krankheitsverlauf höher als bei krzem. 2) Eine Parallelitat zwischen dem BTS-Blutspiegel und der Müdigkeit bestand, besonders war er bei den Fällen, die durch routine Leberfunktionsproben normal beurteilt wurden und in denen über Müdigkeit geklagt wurde, erhöht. 3) Eine Korrelation zwischen dem BTS-Blutspiegel und den routine Leberfunktionsproben bestand nicht, doch bei den Fällen mit normalen routine Leberfunktionsproben fiel der BTS-Blutspiegel in 46.5 Prozent der Fälle positiv aus. Es wäre denkbar, dass der BTS-Blutspiegel eine von den routine Leberfunktionsproben nicht ergriffene Seite ausdrticken könnte. 4) Es gab keine Korrelation zwischen dem BTS,Blutspiegel und dem histologischen Befund der Leber. Doch durch Laparoskopie war der erhöhte BTS-Blutspiegel insbesondere bei dem Ⅱ. und IV. Typus der grossen weissen Leber festgestellt worden. 5) Weil L·BTS in Fällen erhöhter V-BTS (d. h. BTS im Blut) höher war als V-BTS bzw. A-BTS, ausserdem die engste Beziehung von L-BTS/ABTS- Quotienten zum V-BTS-Spiegel (d. h. der BTS-Blutspigel) bestand, wurde bestätigt, dass die erhöhte BTS im Blut bei Leberkrankheiten aus Leber stammt. Der BTS-Blutspiegel spiegelt nämlich den BTS-Stoffwechsel in der Leber wider. 6) Der BTS-Stoffwechsel in der Leber stand in engster Beziehung zu der Leberhamodynamik, d. h. zum visceralem Sauerstoffverbrauch, zum geschatzten Leberdurchblutung und zum Lebervenenverschlussdruck.

An experimental study was attempted to make an analysis of the subcortical and brain stem lesion effect on the Metrazol-induced corticogenic epileptic convulsion based on EEG-discharge and EMG-convulsion as indicators. utilizing 42 adult cats. 1. A definite threshold increment of eliciting the seizure was found in the case of bilateral lesion of the Forel H-field. In contrast to it, no variation in the threshold was found in the case of the lesions at the other parts of brain stem, thalamus, red nucleus and its neighborhood, and lenticular nucleus. 2. There was a parallel relation between EEG discharge and convulsion. Dissociation could be obtained in none of the cases. 3. It is, therefore, to be concluded that the Forel H-field is composed of the main axis of cortico-subcortical reverberating circuit and that the lesion causes a decrement of the excitability at cortex and an inhibition of the corticogenic epileptic convulsion.

An electron microscope study was performed on the ultrastructure and developmental process of the Mukai strain of Japanese B encephalitis virus propagated in vitro on porcine kidney stable cells. The virus particle of Japanese B encephalitis is hexagonal in sections and approximately 40 mμ in the maximum diameter, composed of an outer membrane, 20Å thick, viroplasm, 30 Å thick and an electron-dense nucleoid, 25 mμ in diameter. The virus particles develop by a budding process on the wall of the cytoplasmic vacuole. Thereafter, virus particles are densely packed in the vacuole usually in random arrangement and rarely in crystalline arrays. The vacuole containing virus particles gradually moves toward the cell surface and liberates the virus particles to the exterior of the cells through a narrow canaliculus. A structure suggestive of incomplete virus particles was also observed.

Ehrlich ascites tumor cells affected by oleic and linoleic acids lose their cytomembrane followed by the leak out of ribosomes. Some cells survived through this treatment when they were transplanted into mouse peritoneal cavity, but they changed their characteristics showing wider and less basophilic cytoplasm and smaller nuclei with dense nuclear chromatin and ambiguous nucleoli. In spite of many attempts, no qualitative changes have been found between normal and cancer cells. Recently, Ishikawa found the specific antigenicity of cancer cell membrane which was common to several strains of canccr cells. Grobstein and coworkers have clarified that pancreatic cells can differentiate in association with neighboring mesenchymal cells, probably getting some information. Their works suggest that the cell differentiation will be induced by mutual association of cells by which the cell will receive some substance acting as the information for differentiation. Taking the works of Ishikawa and his collabolators into consideration, it seems that cancer cells may be unable to differentiate by their defective or incomplete cell membrane through which they cannot associate with neighboring cells and fail to get the information. Almost all of the biological characteristics of cancer cells, immaturity, autonomic growth, invasive and metastatic properties independent from the neighboring cell groups, are well explained or consistent with this view. Recently, we found that the cell membrane can be loosened by some unsaturated fatty acids resulting in the leak-out of ribosomes. In this paper it is demonstrated how the Ehrlich ascites tumor cell affected by fatty acids lose their cytomembrane and the ribosomes and how the cells survived through this treatment show different characteristics from the original ones, taking the appearance more matured cells.

Effects of sodium oleate and bovine serum albumin (BSA) on rat liver mitochondrial function and structure were studied by measuring oxygen uptake, 90° light-scattering, adenosine triphosphatase activity and pyridine nucleotides fluorescence. 1. The low concentration of oleate induced the uncoupling of oxidative phosphorylation and the scattering change of mitochondria. This action of oleate differed from that of oleate at a high concentration which induces the high amplitude swelling with respect to its physiological and biochemical properties. The degrees of reversal swelling (shrinkage) and of oxygen uptake induced by oleate in the presence of Pi and succinate were altered proportionately to the concentration of oleate, and the concentration of oleate to the shrinkage coincided with that of the maximal respiratory release. 2. Antimycin A or 2, 4- dinitrophenol prevented the oleate-induced mitochondrial shrinkage, but the treatment of these agents after prior incubation with Pi and succinate allowed the shrinkage, though the degree was small in its extent compared with that in the absence of inhibitors. On the other hand, oligomycin did not affect the shrinkage with oleate. 3. BSA protected the mitochondrial phosphorylation from the uncoupling action of oleate without showing any effect of its own. A complete reversal could readily be demonstrated by a sufficient amount of BSA from the uncoupling, structural changes, and oxidation of intramitochondrial pyridine nucleotides induced by oleate in a low concentration. 4. The oleate-stimulated latent ATPase activity was proportional to the oleate-induced shrinkage of mitochondria with respect to the concentration of oleate. The latent ATPase was abolished also by the addition of a sufficient amount of BSA. 5. The action of oleate on the phosphorylation sequence of mitochondria was discussed on the basis of the present findings.

For the purpose to reveal the mechanism of uptake and degradation of NAD by cells, the authors conducted the observation on the L cells cultured in the medium containing NAD and the following results have been obtained. 1. NAD in the medium is taken up by the cells in its intact form, reaching about twice the value of the control. 2. The spontaneously degraded products of NAD, nicotinamide and adenine dinucleotide ribose, in the same molar concentration as NAD used in the present experiment, have no effect on the NAD content of L cells. 3. The NAD taken up by the cells is degraded into nicotinamide mononucleotide (NMN) and adenine mononucleotide (AMP) by pyrophosphatase including NADpptase and excreted in the medium. Unexpectedly the ingested NAD is not degraded by NADase in the L cell. 4. L cells metabolize the same amount of NAD as that contained originally in the cell for about ten minutes, as calculated from the amount of NMN excreted in the medium.

Sowohl aus dem Grunde, den Mechanismus des gestörten BTS-Stoffwechsels bei den Leberkrankheiten zu erkennen, als auch Beobachtungen für seine Behandlungen zu machen, wurden die Ein£liisse von Zucker, Thiamin und seinen Derivaten (BTMP, TTFD), Thioctsäure, der Verbindung zwischen dem Derivat von Thiamin und Thioctsaure (TATD), Kalium- und Magnesium-Asparaginat und Glucocorticoiden auf den BTS-Blutspiegel untersucht. Das führte zu folgenden Ergebnissen : 1) Der Anstieg des BTS-Blutspiegcls nach Belastung von Glukose bzw. Sorbit wurde beide Male beobachtet, aber er war nach Sorbit geringer als nach Glukose. Das bedeutet, dass Sorbit die BTS-Oxydation fördert. 2) Während der Anstieg des BTS-Blutspiegels mit Thiamin hydrochlorid nicht gehemmt wurde, wurde er mit Thioctsäure in vielen Fällen gehemmt, insbesondere in Rekonvaleszenz der akuten Hepatitis. 3) Nach der Verabreichung Von BTMP, TTFD und TATD war der BTS-Blutspiegel herabgesetzt, aber ihre Einwirkung war bei den Fällen mit gestörter Leberhämodynamik nicht gut. 4) Ebenso hat Kalium- und Magnesium-Asparaginat ungeFähr im Drittel der Fälle den BTS-Blutspiegel erniedrigt. Aber seine Einwirkung in Fällen mit gestörter Leberhämodynamik war ungünstig. 5) Der BTS-Blutspiegel wurde durch Glucocorticoide erhöht.

1) OX substance showed marked cytotoxicities in cell suspension culture of Yoshida sarcoma cells, celothelioma cells, and Ehrlich ascites tumor cells. It has become clear that the cytotoxicities have two aspects; one, nuclear shrinkage and karyolisis as seen with Carzinophilin and the other, cytoplasmic swelling as seen with Nitromin. 2) OX substance was effective by its contact action on patients with peritonitis carcinomatosa, celothelioma and rectal carcinoma. 3) Esterified OX substance was injected intravenously or intraperitonealy into CBA mice with ascites leukemia. The substance prolonged their life span and inhibited the progression of leukemia. As it was possible to give the substance repeatedly into mouse tail veins in this experiment, in the future, OX substance might become intravenously injectable for the treatment of patients with leukemia and solid malignant tumors.

A fibroblast-inhibiting agent, chloroquine, used in the treatment of animal tumors led to a reasonably good result, and this approach was extended to the treatment of human cancers. Of histologically proven 54 cases, the drug was effective in 38, ineffective in 15, and unknown in one. It proved to be effective in all the patients who were treated for over 2 months with exception of terminal patients. Of the various malignant tumors treated, excellent therapeutic effects were obtained in patients with carcinoma of the lung and bladder. In the cases where the drug was effective there were a decrease of the size of tumors, fall of serum lactic dehydrogenase, increase of necrosis, inhibition of the stroma, as well as improvement of the symptoms and general condition. As to the mechanisms of the drug action, it would be necessary to consider of its anti-inflammatory and humoral effects upon the host in addition to its inhibitory action on the stromal connective tissue of cancers. The present chloroquine treatment appears to have its indication in inoperable cases, and pre- and post-operative cases, and for the prevention of reccurrence of tumors. Studies are currently in progress in our laboratory to discover more potent fibroblastinhibiting agents and on the combined chemotherapy of chloroquine and other anti-turnor agents. We are indebted to the Department of Urology of our University for the generosity to allow us to use the clinical data on patients with cancer of the urinary bladder.

1. For the purpose to clarify the relationship between the structural change and lipid composition of isolated rat liver mitochondria, lipid composition and swelling rate of mitochondria obtained from the rat of 3'-Me-DAB feeding and raised in cold room are measured, and the following results were obtained. 2. The mitochondria obtained from the liver of 3'-Me-DAB-fed rat and of rat raised in cold room show a low rate of swelling by addition of Na-oleate accompanied by the decrease in highly unsaturated fatty acids (C18:3 and C20:3or 4) and with the increase in saturated fatty acids (C16 and C18). 3. Activation energy for the mitochondrial swelling is about 16.2 Kcal in the mitochondria obtained from normal rat liver, but requires 19.7 Kcal in the mitochondria that show a low rate of swelling. The fatty acid composition, especially in glycerophosphatides which occupy about 80 per cent of total lipids, is a structural component of mitochondrial membrane, undergoes the change from former to latter in the following fashion: C16:0 21.73→32.10, C16:1 3.37→2.96, C18:0 25.0→29.75, C18:1 13.75→17.40, C18:2 23.90→16.0 and C20:3 or 4 12.23→1.79. 4. At the time of low rate swelling of mitochondria isolated from 3'-MeDAB- fed rat liver, there could be observed a marked increase of the acetone soluble lipid (simple lipids) in the total liver lipids and in the fatty acid distribution of the acetone-soluble lipids, oleic acid was markedly increased (0.838→3.81%/dry liver), despite the fact that in the acetone-insoluble fractions or in the mitochondria there are no marked changes in the oleic acid contents (1.84→2.56% or 0.212→0.246%/dry liver).

1. The forms of irritation causing inflammation and pain are reviewed, with reference to the significance of histamine, serotonin and bradykinin and in particular to the interrelationship between inflammation and pain. 2. The various types of experimental pain are reviewed and mention is made of the human and animal analgesia test methods derived from them. 3. More detailed descriptions are given of the analgesia test methods used by us, namely: a) Silver nitrate gonarthritis-pain, rat, in which both strong and weak analgesics with an anti-inflammatory action are effective. b) Phenylquinone-induced abdominal pain, mouse, in which all the analgesics and anti inflammatory agents mentioned in this article are effective in a greater or lesser degree. c) Tail-flick and hot-plate tests, mouse, in which the strong analgesics, the weaker analgesics and the anti-inflammatory agents, with the exception of the salicylates, are effective. d) Dental-pain test, guinea pig, which can be used to demonstrate the activity of the various analgesics, including the salicylates and also colchicine, which is not active in any other test. e) Pressure-pain, mouse, in which only the strong analgesics (narcotics) are effective. 4. The action of a large number of analgesics, anti-inflammatory agents and related drugs in the various analgesia-tests and in acute experimental inflammation is presented in tabular form. 5. It is concluded that the use of several pain and inflammation tests is essential for screening both analgesics for special indications (severe, mild pain, pain due to inflammation, etc.) and universal pain-killing drugs.