Steroids Show Stereoelectronic Effect - C&EN Global Enterprise (ACS

Nov 6, 2010 - ... 1961, 39 (25), pp 50–55. DOI: 10.1021/cen-v039n025.p050. Publication Date: June 19, 1961. Copyright © 1961 American Chemical Soci...
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RESEARCH

Steroids Show Stereoelectronic Effect Photo-oxygenations of 2-methyl- and 3-methyl-/\2-cholestenes show importance of steric hindrance and steric alignment Two aspects of the catch-all phrase, steric effects, are a little clearer be­ cause of the work of Dr. Alex Nickon and co-workers at Johns Hopkins Uni­ versity, Baltimore, Md. These as­ pects are just plain physical crowding and the importance of a bond having a precise position in space. The first is steric hindrance, the second is called a stereoelectronic effect. The photosensitized oxygenation of olefins serves as the test reaction. The compounds that the Johns Hopkins chemists use are all cholesterol deriva­ tives that differ only in rings A and B. The angular methyl groups at C-10 and C-13 provide the hindrance, and the steroid's rigidity prescribes the geometry of the bonds. Steric hindrance favors attack from

the under (or alpha) side of the ring. The stereoelectronic effect predicts that axial (perpendicular to the ring) allylic bonds will be more reactive than equatorial ones because they over­ lap more readily with the orbitals of the double bond. This overlap may be important in the photoreaction. Such effects can either augment or oppose each other. Oxygen, a diradical, usually reacts by a free radical chain mechanism. There is very little selectivity, and hy­ droperoxides often react further. By contrast, photochemical reaction of oxygen with a dilute olefin solution in presence of a sensitizing agent fre­ quently gives a specific hydroperoxide without going through a chain mecha­ nism [JACS, 83, 1498 (1961)].

CONFERENCE. Dr. Alex Nickon (center) discusses some olefin oxygenation possi­ bilities with Dr. Joseph DiGiorgio (right) as Norman Schwartz looks on 50

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The current theory is that the sen­ sitizing agent—usually a fluorescent dye—absorbs light, is activated, and complexes with oxygen. Then either this complex reacts with an olefin, or the complex dissociates to give acti­ vated oxygen which, in turn, reacts with the olefin. While their experiments do not ex­ pose either of these paths, Dr. Nickon and Dr. Jehanbux F. Bagli, who is now with Ayerst, McKenna & Harrison Re­ search Laboratories, Montreal, are in­ clined to favor attack by the complex. Some support is given by the steric hindrance that they observe. In the photoreaction, the oxygen at­ tacks one end of the double bond. An allylic hydrogen is removed and the double bond moves over one carbon to form an allyl hydroperoxide. Pre­ vious work on open chain compounds reveals little about the steric require­ ments for the loss of this hydrogen be­ cause the bonds are free to rotate to favorable positions, the chemists say. Dr. Nickon points out, though, that steroids provide a rigid system. A°-Cholestene has two hydrogens allylic to the double bond ( 5 a and

8/?). Both of these hydrogens have bonds that are in good position to over­ lap with the orbitals from the double bond during the reaction. The prod­ uct is the 7a-hydiOperoxide. It results from loss of the 5a-hydrogen. No 6-hydroxy-A 7 -steroid (from loss of the 8/?-hydrogen) is observed. This could be due to hindrance by the angular methyl groups. To test the inertness of the 8/?-hydrogen, the 5 position was blocked with an α-hydroxy group. Prolonged reaction left the molecule unchanged. To define the specificity of the re­ action a little further, Dr. Nickon and Dr. Bagli oxygenated 7a-deutero and

The Stereoelectronic Effect,.. In THEORY

and In PRACTICE

Axial bond to X can overlap with the orbitals from the double bond better than the equatorial bond to Y can and will react more easily.

7/?-deutero cholestérols. In both cases, the 7a-substituent was lost, indicating a possible cyclic mechanism.

The 5a-hydroperoxide was formed in each case. The allylic hydrogens that have been shown to react in these steroids are all axial. Their bonds parallel the orbitals of the double bond rather than the rings. A G -Coprostene differs from AG-cholestene (cholesterol without the 3βhydroxyl and with the double bond at C-6) by having a 5β- rather than

a 5a-hydrogen. This gives the mole­ cule a cis A/B ring juncture. The 5/?-hydrogen is more parallel to ring Β than it is to the orbitals of the double bond. This compound is also inert to extended treatment. The case is still not clear-cut, however. It could be argued, the Johns Hopkins group says, that the oxygen must at­ tack from above the ring since the allylic hydrogen involved is above the

No evidence was found for reac­ tion at C-6 from above. The 10βmethyl hinders approach of the complex; bond alignment aids attack at C-5 and C-7 from below.

ring. This would be hindered by the same ΙΟβ-methyl that screens the 8/?-hydrogen. A critical system was needed that would show the relative importance of crowding and bond alignment. Dr. Nickon and Dr. Joseph DiGiorgio found 2-methyl- and 3-methyl-A 2 cholestenes to be such a system. In both compounds, the allylic hy­ drogen involved comes from the methyl group. The hydrogen can al­ ways get into a favored position by rotation, so its effect is the same in either case. In the 2-methyl com­

pound, attack from above is not fav­ ored since the ΙΟβ-methyl blocks it, and because the bond to the hydroperoxy group in the product will not be parallel to the orbitals of the orig­ inal double bond. Attack from be­ low is favored for the opposite rea­ sons. This prediction is borne out by a six-to-one ratio of attack from below. Approach from above will be hin­ dered again by the 10#-methyl in 3-

methyl-A 2 -cholestene. But, in this case, the forming hydroperoxy bond is parallel to the orbitals of the double bond and should be favored. Attack from below gives an equatorial hydro­ peroxy group and will not be favored. Although final purification is not complete, enough evidence is in to show about a fifty-fifty ratio of prod­ ucts. This shows the importance of both steric hindrance and the stereoelectronic effect. When they operate together, the ratio is six to one; when they oppose, it's a standoff. Implications. The use of oxygen, light, fluorescent dye, and olefins is a striking parallel to the processes in living systems. This reaction, using enzymes rather than light, could be one of the ways that oxygen is used in animals. The parallel is even more pointed with plants: the use of light, the quantity and variety of olefins avail­ able, and the variety of oxygenated materials that plants make. Hydro­ peroxy groups are energy rich and can decompose in many ways. They are easily converted to alcohols, ketones, aldehydes, and epoxides; almost any oxygenated material could have a hy­ droperoxy percursor. This makes them attractive as possible oxidation intermediates in living systems. The reaction also has many possi­ bilities as a synthetic tool, particularly when other functional groups are near. JUNE

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D-Luciferin Synthesis Confirms Structure COLONIAL SE SURFACTANTS

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L-Luciferin also made; it reacts biologically at the same rate as the natural but does not produce light Lightning bugs can breathe easier now that the structure and synthesis of luciferin have been settled by Dr. Emil White and co-workers at Johns Hopkins University, Baltimore, Md. Degradative evidence did not lead to a unique structure. However, their suc­ cessful synthesis does complete the structure proof [JACS, 83, 2402 (1961)]. Luciferin (part of the firefly's light­ ing system) is difficult to isolate and purify. No good solvent was found, the material oxidizes readily, and much of the early work was plagued by racemization. It was difficult to get any quantity of luciferin. Most of what was obtained was being used in biological studies by Dr. William D. McElroy of the university's biology department. About 5 mg. was the most that the chemists had at any one time. An early series of analyses indicated that the material probably was a C1:> compound. But recent analyses of a PHOTO. Dr. William McElroy (seated) and Dr. Emil White ponder a 100 χ photograph (inset) of the first crystal­ line natural luciferin that they were able to obtain

luciferin derivative show that it really is a C n compound. These related dif­ ficulties (purification and analysis) were partly offset by an early recogni­ tion of the similarity of the ultraviolet spectrum to those of benzothiazoles. Clues. The carboxyl was recog­ nized; D-cysteine and an aminophenol were found in the degradation prod­ ucts. The ready oxidizability of the molecule suggested that it might be a dihydro derivative of some aromatic system. On this evidence, Dr. White and Dr. Frank McCapra proposed a structure. Luciferin's intractability and the small quantity available drove Dr. White and Dr. George F. Field to synthesize the postulated structure. Synthesis. First, p-anisidine and ethyl oxalate are condensed. Sulfur is introduced with phosphorus pentasulfide. Ferricyanide oxidation closes the benzothiazole ring. The acid is converted to a nitrile via the ester and amide. The methyl is removed from

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the phenol group with pyridine hydrochloride. Finally, this product is condensed at room temperature (in aqueous methanol) with D-cysteine to produce authentic luciferin. No Light. An unusual feature appeared when L-cysteine was used in the synthesis. The L-luciferin behaved just like the D-isomer, even in biological reactions. Dr. McElroy believes that this is the first example where D and L isomers react at the same rate in biological systems. Even more peculiar, the reaction of L-luciferin with the enzyme luciferase, ATP, and oxygen doesn't produce light. How the D-isomer produces light is still a mystery. The broad band emission centering around 565 millimicrons corresponds to an average energy of 50 kilocalories with some of the emission as high as 60 kilocalories. Analytical Tool. D-Luciferin (with enzyme) is very useful in analyzing adenosine t r i p h o s p h a t e (ATP). When a substance containing ATP is added to an aqueous extract of firefly lanterns (which contains D-luciferin), typical firefly light is emitted. The quantum yield is 100% (one luciferin molecule gives one quantum). Measuring the light that's emitted then gives the amount of ATP present. Solutions down to 10 - 1 1 molar can be analyzed. One microgram of ATP per milliliter is analyzed routinely. ATP's involvement in most living material makes the D-luciferin-enzyme system a potent tool for biochemists. This analysis also has severely taxed the firefly population. About 2000 fireflies are needed to produce 1 milligram of D-luciferin. Dr. McElroy has been buying them from school age groups for 25 cents a hundred since 1948. Contests were organized and bonuses given to the winning teams. The average yearly take was about 700,000 fireflies. The synthesis of D-luciferin will reduce the need for the summer collections because fewer fireflies will be needed to supply the demand for the enzyme, luciferase.

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