Division of Psychotherapy: Outgoing Executive Board, August 29, 1968, San Francisco, California

1968 ◽  
PEDIATRICS ◽  
1950 ◽  
Vol 5 (3) ◽  
pp. 504-551

A meeting of the Executive Board of the American Academy of Pediatrics was held at the Palace Hotel, San Francisco, Calif., on Friday, Nov. 11, 1949. It was called to order at 10:00 a.m. by the President, Dr. Warren R. Sisson. There were present Drs. Sisson, Shaw, Barba, Beaven, Bost, London, Munns, McElhenney, Stringfield, Wishropp, Grulee, Martmer, Pease and Bakwin. The first order of business was the consideration of applicants: the following were approved. This gives me an opportunity to speak briefly of the Executive Board meetings. They offer the greatest opportunity for considered opinion and guidance of Academy affairs that exists in our organization. As your President, I have been greatly impressed by the good balance of the membership its great sense of responsibility to the Academy and its untiring efforts. I feel that the deliberations or minutes of the Executive Board should be distributed to the members as early as possible while interest still exists in current discussions. One cannot overemphasize the importance of putting the deliberations of the Board out in an attractive format to encourage greater publicity. In spite of my New England streak of economy, I would earnestly recommend quarterly meetings of the Board and placing more emphasis upon the policies of the Academy in planning our activities in the broad field of public health. I do not see how this can be done without frequent meetings and assignment of special subjects to special committees of the governing body. In this connection I recommend that the Executive Board be thoroughly conversant with the finances of the Academy and appoint the Budget Committee from its membership. The second subject which I would like to bring to your attention is that of public relations. Early in my term of office, you voted to appoint a committee to investigate this subject. It has seemed to your President one of the important activities of the Academy.


PEDIATRICS ◽  
1950 ◽  
Vol 5 (1) ◽  
pp. 145-146
Author(s):  
EDWARD B. SHAW

The President and the Executive Board send their greetings to the membership of the Academy of Pediatrics for the new year. This column will appear irregularly from time to time in an effort to keep the membership apprised of developments which affect the Academy and which must be considered by the Executive Board. The President and the District Chairmen are elective officers of the Academy and in the true sense of democratic representation can only attempt to interpret the opinions of the membership in their action on problems which arise. American medicine is now confronted with many problems upon which neither the individual nor the organization can avoid taking a position. The action of your executive officers must be predicated upon the expression of opinion by the membership. It is hoped that you will keep your officers informed of individual and group opinions upon controversial issues in order to guide their action. The columns of Pediatrics IATRICS are open to the membership in "The Pediatrician and the Public" but it is most desirable that you communicate with your officers directly for their information. The San Francisco session was astonishingly well attended considering the handicap which distance imposed upon many of the members. I should be remiss in not expressing the pleasure of the local Fellows that so many should have come so far and contributed so much. Dr. Edgar E. Martmer and his Program Committee are to be congratulated not only because of the excellence of the program but also because they were able to effect last minute substitutions for participants who, because of illness, were unable to attend, without impairing the structure of the meeting.


Author(s):  
László G. Kömüves

Light microscopic immunohistochemistry based on the principle of capillary action staining is a widely used method to localize antigens. Capillary action immunostaining, however, has not been tested or applied to detect antigens at the ultrastructural level. The aim of this work was to establish a capillary action staining method for localization of intracellular antigens, using colloidal gold probes.Post-embedding capillary action immunocytochemistry was used to detect maternal IgG in the small intestine of newborn suckling piglets. Pieces of the jejunum of newborn piglets suckled for 12 h were fixed and embedded into LR White resin. Sections on nickel grids were secured on a capillary action glass slide (100 μm wide capillary gap, Bio-Tek Solutions, Santa Barbara CA, distributed by CMS, Houston, TX) by double sided adhesive tape. Immunolabeling was performed by applying reagents over the grids using capillary action and removing reagents by blotting on filter paper. Reagents for capillary action staining were from Biomeda (Foster City, CA). The following steps were performed: 1) wet the surface of the sections with automation buffer twice, 5 min each; 2) block non-specific binding sites with tissue conditioner, 10 min; 3) apply first antibody (affinity-purified rabbit anti-porcine IgG, Sigma Chem. Co., St. Louis, MO), diluted in probe diluent, 1 hour; 4) wash with automation buffer three times, 5 min each; 5) apply gold probe (goat anti-rabbit IgG conjugated to 10 nm colloidal gold, Zymed Laboratories, South San Francisco, CA) diluted in probe diluent, 30 min; 6) wash with automation buffer three times, 5 min each; 7) post-fix with 5% glutaraldehyde in PBS for 10 min; 8) wash with PBS twice, 5 min each; 9) contrast with 1% OSO4 in PBS for 15 min; 10) wash with PBS followed by distilled water for5 min each; 11) stain with 2% uranyl acetate for 10 min; 12) stain with lead citrate for 2 min; 13) wash with distilled water three times, 1 min each. The glass slides were separated, and the grids were air-dried, then removed from the adhesive tape. The following controls were used to ensure the specificity of labeling: i) omission of the first antibody; ii) normal rabbit IgG in lieu of first antibody; iii) rabbit anti-porcine IgG absorbed with porcine IgG.


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